Gene expression markers for breast cancer prognosis

ABSTRACT

The present invention provides gene sets the expression of which is important in the diagnosis and/or prognosis of breast cancer.

[0001] This application claims priority under 35 U.S.C. § 119(e) to provisional application Serial No. 60/440,661 filed on Jan. 15, 2003, the entire disclosure of which is hereby expressly incorporated by reference.

BACKGROUND OF THE INVENTION

[0002] 1. Field of the Invention

[0003] The present invention provides genes and gene sets the expression of which is important in the diagnosis and/or prognosis of breast cancer.

[0004] 2. Description of the Related Art

[0005] Oncologists have a number of treatment options available to them, including different combinations of chemotherapeutic drugs that are characterized as “standard of care,” and a number of drugs that do not carry a label claim for particular cancer, but for which there is evidence of efficacy in that cancer. Best likelihood of good treatment outcome requires that patients be assigned to optimal available cancer treatment, and that this assignment be made as quickly as possible following diagnosis.

[0006] Currently, diagnostic tests used in clinical practice are single analyte, and therefore do not capture the potential value of knowing relationships between dozens of different markers. Moreover, diagnostic tests are frequently not quantitative, relying on immunohistochemistry. This method often yields different results in different laboratories, in part because the reagents are not standardized, and in part because the interpretations are subjective and cannot be easily quantified. RNA-based tests have not often been used because of the problem of RNA degradation over time and the fact that it is difficult to obtain fresh tissue samples from patients for analysis. Fixed paraffin-embedded tissue is more readily available and methods have been established to detect RNA in fixed tissue. However, these methods typically do not allow for the study of large numbers of genes (DNA or RNA) from small amounts of material. Thus, traditionally fixed tissue has been rarely used other than for immunohistochemistry detection of proteins.

[0007] Recently, several groups have published studies concerning the classification of various cancer types by microarray gene expression analysis (see, e.g. Golub et al., Science 286:531-537 (1999); Bhattacharjae et al., Proc. Natl. Acad. Sci. USA 98:13790-13795 (2001); Chen-Hsiang et al., Bioinformatics 17 (Suppl. 1):S316-S322 (2001); Ramaswamy et al., Proc. Natl. Acad. Sci. USA 98:15149-15154 (2001)). Certain classifications of human breast cancers based on gene expression patterns have also been reported (Martin et al., Cancer Res. 60:2232-2238 (2000); West et al., Proc. Natl. Acad. Sci. USA 98:11462-11467 (2001); Sorlie et al., Proc. Natl. Acad. Sci. USA 98:10869-10874 (2001); Yan et al., Cancer Res. 61:8375-8380 (2001)). However, these studies mostly focus on improving and refining the already established classification of various types of cancer, including breast cancer, and generally do not provide new insights into the relationships of the differentially expressed genes, and do not link the findings to treatment strategies in order to improve the clinical outcome of cancer therapy.

[0008] Although modern molecular biology and biochemistry have revealed hundreds of genes whose activities influence the behavior of tumor cells, state of their differentiation, and their sensitivity or resistance to certain therapeutic drugs, with a few exceptions, the status of these genes has not been exploited for the purpose of routinely making clinical decisions about drug treatments. One notable exception is the use of estrogen receptor (ER) protein expression in breast carcinomas to select patients to treatment with anti-estrogen drugs, such as tamoxifen. Another exceptional example is the use of ErbB2 (Her2) protein expression in breast carcinomas to select patients with the Her2 antagonist drug Herceptin® (Genentech, Inc., South San Francisco, Calif.).

[0009] Despite recent advances, the challenge of cancer treatment remains to target specific treatment regimens to pathogenically distinct tumor types, and ultimately personalize tumor treatment in order to maximize outcome. Hence, a need exists for tests that simultaneously provide predictive information about patient responses to the variety of treatment options. This is particularly true for breast cancer, the biology of which is poorly understood. It is clear that the classification of breast cancer into a few subgroups, such as ErbB2+subgroup, and subgroups characterized by low to absent gene expression of the estrogen receptor (ER) and a few additional transcriptional factors (Perou et al., Nature 406:747-752 (2000)) does not reflect the cellular and molecular heterogeneity of breast cancer, and does not allow the design of treatment strategies maximizing patient response.

SUMMARY OF THE INVENTION

[0010] The present invention provides a set of genes, the expression of which has prognostic value, specifically with respect to disease-free survival.

[0011] The present invention accommodates the use of archived paraffin-embedded biopsy material for assay of all markers in the set, and therefore is compatible with the most widely available type of biopsy material. It is also compatible with several different methods of tumor tissue harvest, for example, via core biopsy or fine needle aspiration. Further, for each member of the gene set, the invention specifies oligonucleotide sequences that can be used in the test.

[0012] In one aspect, the invention concerns a method of predicting the likelihood of long-term survival of a breast cancer patient without the recurrence of breast cancer, comprising determining the expression level of one or more prognostic RNA transcripts or their expression products in a breast cancer tissue sample obtained from the patient, normalized against the expression level of all RNA transcripts or their products in the breast cancer tissue sample, or of a reference set of RNA transcripts or their expression products, wherein the prognostic RNA transcript is the transcript of one or more genes selected from the group consisting of: TP53BP2, GRB7, PR, CD68, Bc12, KRT14, IRS1, CTSL, EstR1, Chk1, IGFBP2, BAG1, CEGP1, STK15, GSTM1, FHIT, RIZ1, AIB1, SURV, BBC3, IGF1R, p27, GATA3, ZNF217, EGFR, CD9, MYBL2, HIF1α, pS2, ErbB3, TOP2B, MDM2, RAD51C, KRT19, TS, Her2, KLK10, β-Catenin, γ-Catenin, MCM2, PI3KC2A, IGF1, TBP, CCNB1, FBXO5, and DR5,

[0013] wherein expression of one or more of GRB7, CD68, CTSL, Chk1, AIB1, CCNB1, MCM2, FBXO5, Her2, STK15, SURV, EGFR, MYBL2, HIF1α, and TS indicates a decreased likelihood of long-term survival without breast cancer recurrence, and

[0014] the expression of one or more of TP53BP2, PR, Bc12, KRT14, EstR1, IGFBP2, BAG1, CEGP1, KLK10, β-Catenin, γ-Catenin, DR5, PI3KCA2, RAD51C, GSTM1, FHIT, RIZ1, BBC3, TBP, p27, IRS1, IGF1R, GATA3, ZNF217, CD9, pS2, ErbB3, TOP2B, MDM2, IGF1, and KRT19 indicates an increased likelihood of long-term survival without breast cancer recurrence.

[0015] In a particular embodiment, the expression levels of at least two, or at least 5, or at least 10, or at least 15 of the prognostic RNA transcripts or their expression products are determined. In another embodiment, the method comprises the determination of the expression levels of all prognostic RNA transcripts or their expression products.

[0016] In another particular embodiment, the breast cancer is invasive breast carcinoma.

[0017] In a further embodiment, RNA is isolated from a fixed, wax-embedded breast cancer tissue specimen of the patient. Isolation may be performed by any technique known in the art, for example from core biopsy tissue or fine needle aspirate cells.

[0018] In another aspect, the invention concerns an array comprising polynucleotides hybridizing to two or more of the following genes: α-Catenin, AIB1, AKT1, AKT2, β-actin, BAG1, BBC3, Bc12, CCNB1, CCND1, CD68, CD9, CDH1, CEGP1, Chk1, CIAP1, cMet.2, Contig 27882, CTSL, DR5, EGFR, EIF4E, EPHX1, ErbB3, EstR1, FBXO5, FHIT1 FRP1, GAPDH, GATA3, G-Catenin, GRB7, GRO1, GSTM1, GUS, HER2, HIF1A, HNF3A, IGF1R, IGFBP2, KLK10, KRT14, KRT17, KRT18, KRT19, KRT5, Maspin, MCM2, MCM3, MDM2, MMP9, MTA1, MYBL2, P14ARF, p27, P53, PI3KC2A, PR, PRAME, pS2, RAD51C, 3RB1, RIZ1, STK15, STMY3, SURV, TGFA, TOP2B, TP53BP2, TRAIL, TS, upa, VDR, VEGF, and ZNF217.

[0019] In particular embodiments, the array comprises polynucleotides hybridizing to at least 3, or at least 5, or at least 10, or at least 15, or at least 20, or all of the genes listed above.

[0020] In another specific embodiment, the array comprises polynucleotides hybridizing to the following genes: TP53BP2, GRB7, PR, CD68, Bc12, KRT14, IRS1, CTSL, EstR1, Chk1, IGFBP2, BAG1, CEGP1, STK15, GSTM1, FHIT, RIZ1, AIB1, SURV, BBC3, IGF1R, p27, GATA3, ZNF217, EGFR, CD9, MYBL2, HIF1α, pS2, RIZ1, ErbB3, TOP2B, MDM2, RAD51C, KRT19, TS, Her2, KLK10, β-Catenin, γ-Catenin, MCM2, PI3KC2A, IGF1, TBP, CCNB1, FBXO5 and DR5.

[0021] The polynucleotides can be cDNAs, or oligonucleotides, and the solid surface on which they are displayed may, for example, be glass.

[0022] In another aspect, the invention concerns a method of predicting the likelihood of long-term survival of a patient diagnosed with invasive breast cancer, without the recurrence of breast cancer, comprising the steps of:

[0023] (1) determining the expression levels of the RNA transcripts or the expression products of genes or a gene set selected from the group consisting of

[0024] (a) TP53BP2, Bc12, BAD, EPHX1, PDGFRβ, DIABLO, XIAP, YB1, CA9, and KRT8;

[0025] (b) GRB7, CD68, TOP2A, Bc12, DIABLO, CD3, ID1, PPM1D, MCM6, and WISP1;

[0026] (c) PR, TP53BP2, PRAME, DIABLO, CTSL, IGFBP2, TIMP1, CA9, MMP9, and COX2;

[0027] (d) CD68, GRB7, TOP2A, Bc12, DIABLO, CD3, ID1, PPM1D, MCM6, and WISP1;

[0028] (e) Bc12, TP53BP2, BAD, EPHX1, PDGFRβ, DIABLO, XIAP, YB1, CA9, and KRT8;

[0029] (f) KRT14, KRT5, PRAME, TP53BP2, GUS1, AIB1, MCM3, CCNE1, MCM6, and ID1;

[0030] (g) PRAME, TP53BP2, EstR1, DIABLO, CTSL, PPM1D, GRB7, DAPK1, BBC3, and VEGFB;

[0031] (h) CTSL2, GRB7, TOP2A, CCNB1, Bc12, DIABLO, PRAME, EMS1, CA9, and EpCAM;

[0032] (i) EstR1, TP53BP2, PRAME, DIABLO, CTSL, PPM1D, GRB7, DAPK1, BBC3, and VEGFB;

[0033] (k) Chk1, PRAME, TP53BP2, GRB7, CA9, CTSL, CCNB1, TOP2A, tumor size, and IGFBP2;

[0034] (l) IGFBP2, GRB7, PRAME, DIABLO, CTSL, β-Catenin, PPM1D, Chk1, WISP1, and LOT1;

[0035] (m) HER2, TP53BP2, Bc12, DIABLO, TIMP1, EPHX1, TOP2A, TRAIL, CA9, and AREG;

[0036] (n) BAG1, TP53BP2, PRAME, IL6, CCNB1, PAI1, AREG, tumor size, CA9, and Ki67;

[0037] (o) CEGP1, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, STK15, and AKT2, and FGF18;

[0038] (p) STK15, TP53BP2, PRAME, IL6, CCNE1, AKT2, DIABLO, cMet, CCNE2, and COX2;

[0039] (q) KLK10, EstR1, TP53BP2, PRAME, DIABLO, CTSL, PPM1D, GRB7, DAPK1, and BBC3;

[0040] (r) AIB1, TP53BP2, Bc12, DIABLO, TIMP1, CD3, p53, CA9, GRB7, and EPHX1

[0041] (s) BBC3, GRB7, CD68, PRAME, TOP2A, CCNB1, EPHX1, CTSL GSTM1, and APC;

[0042] (t) CD9, GRB7, CD68, TOP2A, Bc12, CCNB1, CD3, DIABLO, ID1, and PPM1D;

[0043] (w) EGFR, KRT14, GRB7, TOP2A, CCNB1, CTSL, Bc12, TP, KLK10, and CA9;

[0044] (x) HIF1α, PR, DIABLO, PRAME, Chk1, AKT2, GRB7, CCNE1, TOP2A, and CCNB1;

[0045] (y) MDM2, TP53BP2, DIABLO, Bc12, AIB1, TIMP1, CD3, p53, CA9, and HER2;

[0046] (z) MYBL2, TP53BP2, PRAME, IL6, Bc12, DIABLO, CCNE1, EPHX1, TIMP1, and CA9;

[0047] (aa) p27, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, STK15, AKT2, and ID1;

[0048] (ab) RAD51, GRB7, CD68, TOP2A, CIAP2, CCNB1, BAG1, IL6, FGFR1, and TP53BP2;

[0049] (ac) SURV, GRB7, TOP2A, PRAME, CTSL, GSTM1, CCNB1, VDR, CA9; and CCNE2;

[0050] (ad) TOP2B, TP53BP2, DIABLO, Bc12, TIMP1, AIB1, CA9, p53, KRT8, and BAD;

[0051] (ae) ZNF217, GRB7, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, APC4, and β-Catenin,

[0052] in a breast cancer tissue sample obtained from the patient, normalized against the expression levels of all RNA transcripts or their expression products in said breast cancer tissue sample, or of a reference set of RNA transcripts or their products;

[0053] (2) subjecting the data obtained in step (1) to statistical analysis; and

[0054] (3) determining whether the likelihood of said long-term survival has increased or decreased.

[0055] In a further aspect, the invention concerns a method of predicting the likelihood of long-term survival of a patient diagnosed with estrogen receptor (ER)-positive invasive breast cancer, without the recurrence of breast cancer, comprising the steps of:

[0056] (1) determining the expression levels of the RNA transcripts or the expression products of genes of a gene set selected from the group consisting of CD68; CTSL; FBXO5; SURV; CCNB1; MCM2; Chk1; MYBL2; HIF1A; cMET; EGFR; TS; STK15, IGFR1; BC12; HNF3A; TP53BP2; GATA3; BBC3; RAD51C; BAG1; IGFBP2; PR; CD9; RB1; EPHX1; CEGP1; TRAIL; DR5; p27; p53; MTA; RIZ1; ErbB3; TOP2B; EIF4E, wherein expression of the following genes in ER-positive cancer is indicative of a reduced likelihood of survival without cancer recurrence following surgery: CD68; CTSL; FBXO5; SURV; CCNB1; MCM2; Chk1; MYBL2; HIF1A; cMET; EGFR; TS; STK15, and wherein expression of the following genes is indicative of a better prognosis for survival without cancer recurrence following surgery: IGFR1; BC12; HNF3A; TP53BP2; GATA3; BBC3; RAD51C; BAG1; IGFBP2; PR; CD9; RB1; EPHX1; CEGP1; TRAIL; DR5; p27; p53; MTA; RIZ1; ErbB3; TOP2B; EIF4E.

[0057] (2) subjecting the data obtained in step (1) to statistical analysis; and

[0058] (3) determining whether the likelihood of said long-term survival has increased or decreased.

[0059] In yet another aspect, the invention concerns a method of predicting the likelihood of long-term survival of a patient diagnosed with estrogen receptor (ER)-negative invasive breast cancer, without the recurrence of breast cancer, comprising determining the expression levels of the RNA transcripts or the expression products of genes of the gene set CCND1; UPA; HNF3A; CDH1; Her2; GRB7; AKT1; STMY3; α-Catenin; VDR; GRO1; KT14; KLK10; Maspin, TGFα, and FRP1, wherein expression of the following genes is indicative of a reduced likelihood of survival without cancer recurrence: CCND1; UPA; HNF3A; CDH1; Her2; GRB7; AKT1; STMY3; α-Catenin; VDR; GRO1, and wherein expression of the following genes is indicative of a better prognosis for survival without cancer recurrence: KT14; KLK10; Maspin, TGFα, and FRP1.

[0060] In a different aspect, the invention concerns a method of preparing a personalized genomics profile for a patient, comprising the steps of:

[0061] (a) subjecting RNA extracted from a breast tissue obtained from the patient to gene expression analysis;

[0062] (b) determining the expression level of one or more genes selected from the breast cancer gene set listed in any one of Tables 1-5, wherein the expression level is normalized against a control gene or genes and optionally is compared to the amount found in a breast cancer reference tissue set; and

[0063] (c) creating a report summarizing the data obtained by the gene expression analysis.

[0064] The report may, for example, include prediction of the likelihood of long term survival of the patient and/or recommendation for a treatment modality of said patient.

[0065] In a further aspect, the invention concerns a method for amplification of a gene listed in Tables 5A and B by polymerase chain reaction (PCR), comprising performing said PCR by using an amplicon listed in Tables 5A and B and a primer-probe set listed in Tables 6A-F.

[0066] In a still further aspect, the invention concerns a PCR amplicon listed in Tables 5A and B.

[0067] In yet another aspect, the invention concerns a PCR primer-probe set listed in Tables 6A-F.

[0068] The invention further concerns a prognostic method comprising:

[0069] (a) subjecting a sample comprising breast cancer cells obtained from a patient to quantitative analysis of the expression level of the RNA transcript of at least one gene selected from the group consisting of GRB7, CD68, CTSL, Chk1, AIB1, CCNB1, MCM2, FBXO5, Her2, STK15, SURV, EGFR, MYBL2, HIF1α, and TS, or their product, and

[0070] (b) identifying the patient as likely to have a decreased likelihood of long-term survival without breast cancer recurrence if the normalized expression levels of the gene or genes, or their products, are elevated above a defined expression threshold.

[0071] In a different aspect, the invention concerns a prognostic method comprising:

[0072] (a) subjecting a sample comprising breast cancer cells obtained from a patient to quantitative analysis of the expression level of the RNA transcript of at least one gene selected from the group consisting of TP53BP2, PR, Bc12, KRT14, EstR1, IGFBP2, BAG1, CEGP1, KLK10, β-Catenin, γ-Catenin, DR5, PI3KCA2, RAD51C, GSTM1, FHIT, RIZ1, BBC3, TBP, p27, IRS1, IGF1R, GATA3, ZNF217, CD9, pS2, ErbB3, TOP2B, MDM2, IGF1, and KRT19, and

[0073] (b) identifying the patient as likely to have an increased likelihood of long-term survival without breast cancer recurrence if the normalized expression levels of the gene or genes, or their products, are elevated above a defined expression threshold.

[0074] The invention further concerns a kit comprising one or more of (1) extraction buffer/reagents and protocol; (2) reverse transcription buffer/reagents and protocol; and (3) qPCR buffer/reagents and protocol suitable for performing any of the foregoing methods.

BRIEF DESCRIPTION OF THE DRAWINGS

[0075] Table 1 is a list of genes, expression of which correlate with breast cancer survival. Results from a retrospective clinical trial. Binary statistical analysis.

[0076] Table 2 is a list of genes, expression of which correlates with breast cancer survival in estrogen receptor (ER) positive patients. Results from a retrospective clinical trial. Binary statistical analysis.

[0077] Table 3 is a list of genes, expression of which correlates with breast cancer survival in estrogen receptor (ER) negative patients. Results from a retrospective clinical trial. Binary statistical analysis.

[0078] Table 4 is a list of genes, expression of which correlates with breast cancer survival. Results from a retrospective clinical trial. Cox proportional hazards statistical analysis.

[0079] Tables 5A and B show a list of genes, expression of which correlate with breast cancer survival. Results from a retrospective clinical trial. The table includes accession numbers for the genes, and amplicon sequences used for PCR amplification.

[0080] Tables 6A-6F The table includes sequences for the forward and reverse primers (designated by “f” and “r”, respectively) and probes (designated by “p”) used for PCR amplification of the amplicons listed in Tables 5A-B.

DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT

[0081] A. Definitions

[0082] Unless defined otherwise, technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Singleton et al., Dictionary of Microbiology and Molecular Biology 2nd ed., J. Wiley & Sons (New York, N.Y. 1994), and March, Advanced Organic Chemistry Reactions, Mechanisms and Structure 4th ed., John Wiley & Sons (New York, N.Y. 1992), provide one skilled in the art with a general guide to many of the terms used in the present application.

[0083] One skilled in the art will recognize many methods and materials similar or equivalent to those described herein, which could be used in the practice of the present invention. Indeed, the present invention is in no way limited to the methods and materials described. For purposes of the present invention, the following terms are defined below.

[0084] The term “microarray” refers to an ordered arrangement of hybridizable array elements, preferably polynucleotide probes, on a substrate.

[0085] The term “polynucleotide,” when used in singular or plural, generally refers to any polyribonucleotide or polydeoxribonucleotide, which may be unmodified RNA or DNA or modified RNA or DNA. Thus, for instance, polynucleotides as defined herein include, without limitation, single- and double-stranded DNA, DNA including single- and double-stranded regions, single- and double-stranded RNA, and RNA including single- and double-stranded regions, hybrid molecules comprising DNA and RNA that may be single-stranded or, more typically, double-stranded or include single- and double-stranded regions. In addition, the term “polynucleotide” as used herein refers to triple-stranded regions comprising RNA or DNA or both RNA and DNA. The strands in such regions may be from the same molecule or from different molecules. The regions may include all of one or more of the molecules, but more typically involve only a region of some of the molecules. One of the molecules of a triple-helical region often is an oligonucleotide. The term “polynucleotide” specifically includes cDNAs. The term includes DNAs (including cDNAs) and RNAs that contain one or more modified bases. Thus, DNAs or RNAs with backbones modified for stability or for other reasons are “polynucleotides” as that term is intended herein. Moreover, DNAs or RNAs comprising unusual bases, such as inosine, or modified bases, such as tritiated bases, are included within the term “polynucleotides” as defined herein. In general, the term “polynucleotide” embraces all chemically, enzymatically and/or metabolically modified forms of unmodified polynucleotides, as well as the chemical forms of DNA and RNA characteristic of viruses and cells, including simple and complex cells.

[0086] The term “oligonucleotide” refers to a relatively short polynucleotide, including, without limitation, single-stranded deoxyribonucleotides, single- or double-stranded ribonucleotides, RNA:DNA hybrids and double-stranded DNAs. Oligonucleotides, such as single-stranded DNA probe oligonucleotides, are often synthesized by chemical methods, for example using automated oligonucleotide synthesizers that are commercially available. However, oligonucleotides can be made by a variety of other methods, including in vitro recombinant DNA-mediated techniques and by expression of DNAs in cells and organisms.

[0087] The terms “differentially expressed gene,” “differential gene expression” and their synonyms, which are used interchangeably, refer to a gene whose expression is activated to a higher or lower level in a subject suffering from a disease, specifically cancer, such as breast cancer, relative to its expression in a normal or control subject. The terms also include genes whose expression is activated to a higher or lower level at different stages of the same disease. It is also understood that a differentially expressed gene may be either activated or inhibited at the nucleic acid level or protein level, or may be subject to alternative splicing to result in a different polypeptide product. Such differences may be evidenced by a change in mRNA levels, surface expression, secretion or other partitioning of a polypeptide, for example. Differential gene expression may include a comparison of expression between two or more genes or their gene products, or a comparison of the ratios of the expression between two or more genes or their gene products, or even a comparison of two differently processed products of the same gene, which differ between normal subjects and subjects suffering from a disease, specifically cancer, or between various stages of the same disease. Differential expression includes both quantitative, as well as qualitative, differences in the temporal or cellular expression pattern in a gene or its expression products among, for example, normal and diseased cells, or among cells which have undergone different disease events or disease stages. For the purpose of this invention, “differential gene expression” is considered to be present when there is at least an about two-fold, preferably at least about four-fold, more preferably at least about six-fold, most preferably at least about ten-fold difference between the expression of a given gene in normal and diseased subjects, or in various stages of disease development in a diseased subject.

[0088] The phrase “gene amplification” refers to a process by which multiple copies of a gene or gene fragment are formed in a particular cell or cell line. The duplicated region (a stretch of amplified DNA) is often referred to as “amplicon.” Usually, the amount of the messenger RNA (mRNA) produced, i.e., the level of gene expression, also increases in the proportion of the number of copies made of the particular gene expressed.

[0089] The term “diagnosis” is used herein to refer to the identification of a molecular or pathological state, disease or condition, such as the identification of a molecular subtype of head and neck cancer, colon cancer, or other type of cancer.

[0090] The term “prognosis” is used herein to refer to the prediction of the likelihood of cancer-attributable death or progression, including recurrence, metastatic spread, and drug resistance, of a neoplastic disease, such as breast cancer.

[0091] The term “prediction” is used herein to refer to the likelihood that a patient will respond either favorably or unfavorably to a drug or set of drugs, and also the extent of those responses, or that a patient will survive, following surgical removal or the primary tumor and/or chemotherapy for a certain period of time without cancer recurrence. The predictive methods of the present invention can be used clinically to make treatment decisions by choosing the most appropriate treatment modalities for any particular patient. The predictive methods of the present invention are valuable tools in predicting if a patient is likely to respond favorably to a treatment regimen, such as surgical intervention, chemotherapy with a given drug or drug combination, and/or radiation therapy, or whether long-term survival of the patient, following sugery and/or termination of chemotherapy or other treatment modalities is likely.

[0092] The term “long-term” survival is used herein to refer to survival for at least 3 years, more preferably for at least 8 years, most preferably for at least 10 years following surgery or other treatment.

[0093] The term “tumor,” as used herein, refers to all neoplastic cell growth and proliferation, whether malignant or benign, and all pre-cancerous and cancerous cells and tissues.

[0094] The terms “cancer” and “cancerous” refer to or describe the physiological condition in mammals that is typically characterized by unregulated cell growth. Examples of cancer include but are not limited to, breast cancer, colon cancer, lung cancer, prostate cancer, hepatocellular cancer, gastric cancer, pancreatic cancer, cervical cancer, ovarian cancer, liver cancer, bladder cancer, cancer of the urinary tract, thyroid cancer, renal cancer, carcinoma, melanoma, and brain cancer.

[0095] The “pathology” of cancer includes all phenomena that compromise the well-being of the patient. This includes, without limitation, abnormal or uncontrollable cell growth, metastasis, interference with the normal functioning of neighboring cells, release of cytokines or other secretory products at abnormal levels, suppression or aggravation of inflammatory or immunological response, neoplasia, premalignancy, malignancy, invasion of surrounding or distant tissues or organs, such as lymph nodes, etc.

[0096] “Stringency” of hybridization reactions is readily determinable by one of ordinary skill in the art, and generally is an empirical calculation dependent upon probe length, washing temperature, and salt concentration. In general, longer probes require higher temperatures for proper annealing, while shorter probes need lower temperatures. Hybridization generally depends on the ability of denatured DNA to reanneal when complementary strands are present in an environment below their melting temperature. The higher the degree of desired homology between the probe and hybridizable sequence, the higher the relative temperature which can be used. As a result, it follows that higher relative temperatures would tend to make the reaction conditions more stringent, while lower temperatures less so. For additional details and explanation of stringency of hybridization reactions, see Ausubel et al., Current Protocols in Molecular Biology, Wiley Interscience Publishers, (1995).

[0097] “Stringent conditions” or “high stringency conditions”, as defined herein, typically: (1) employ low ionic strength and high temperature for washing, for example 0.015 M sodium chloride/0.0015 M sodium citrate/0.1% sodium dodecyl sulfate at 50° C.; (2) employ during hybridization a denaturing agent, such as formamide, for example, 50% (v/v) formamide with 0.1% bovine serum albumin/0.1% Ficoll/0.1% polyvinylpyrrolidone/50 mM sodium phosphate buffer at pH 6.5 with 750 mM sodium chloride, 75 mM sodium citrate at 42° C.; or (3) employ 50% formamide, 5×SSC (0.75 M NaCl, 0.075 M sodium citrate), 50 mM sodium phosphate (pH 6.8), 0.1% sodium pyrophosphate, 5× Denhardt's solution, sonicated salmon sperm DNA (50 μg/ml), 0.1% SDS, and 10% dextran sulfate at 42° C., with washes at 42° C. in 0.2×SSC (sodium chloride/sodium citrate) and 50% formamide at 55° C., followed by a high-stringency wash consisting of 0.1×SSC containing EDTA at 55° C.

[0098] “Moderately stringent conditions” may be identified as described by Sambrook et al., Molecular Cloning: A Laboratory Manual, New York: Cold Spring Harbor Press, 1989, and include the use of washing solution and hybridization conditions (e.g., temperature, ionic strength and % SDS) less stringent that those described above. An example of moderately stringent conditions is overnight incubation at 37° C. in a solution comprising: 20% formamide, 5×SSC (150 mM NaCl, 15 mM trisodium citrate), 50 mM sodium phosphate (pH 7.6), 5× Denhardt's solution, 10% dextran sulfate, and 20 mg/ml denatured sheared salmon sperm DNA, followed by washing the filters in 1×SSC at about 37-50° C. The skilled artisan will recognize how to adjust the temperature, ionic strength, etc. as necessary to accommodate factors such as probe length and the like.

[0099] In the context of the present invention, reference to “at least one,” “at least two,” “at least five,” etc. of the genes listed in any particular gene set means any one or any and all combinations of the genes listed.

[0100] The terms “expression threshold,” and “defined expression threshold” are used interchangeably and refer to the level of a gene or gene product in question above which the gene or gene product serves as a predictive marker for patient survival without cancer recurrence. The threshold is defined experimentally from clinical studies such as those described in the Example below. The expression threshold can be selected either for maximum sensitivity, or for maximum selectivity, or for minimum error. The determination of the expression threshold for any situation is well within the knowledge of those skilled in the art.

[0101] B. Detailed Description

[0102] The practice of the present invention will employ, unless otherwise indicated, conventional techniques of molecular biology (including recombinant techniques), microbiology, cell biology, and biochemistry, which are within the skill of the art. Such techniques are explained fully in the literature, such as, “Molecular Cloning: A Laboratory Manual”, 2^(nd) edition (Sambrook et al., 1989); “Oligonucleotide Synthesis” (M. J. Gait, ed., 1984); “Animal Cell Culture” (R. I. Freshney, ed., 1987); “Methods in Enzymology” (Academic Press, Inc.); “Handbook of Experimental Immunology”, 4^(th) edition (D. M. Weir & C. C. Blackwell, eds., Blackwell Science Inc., 1987); “Gene Transfer Vectors for Mammalian Cells” (J. M. Miller & M. P. Calos, eds., 1987); “Current Protocols in Molecular Biology” (F. M. Ausubel et al., eds., 1987); and “PCR: The Polymerase Chain Reaction”, (Mullis et al., eds., 1994).

[0103] 1. Gene Expression Profiling

[0104] In general, methods of gene expression profiling can be divided into two large groups: methods based on hybridization analysis of polynucleotides, and methods based on sequencing of polynucleotides. The most commonly used methods known in the art for the quantification of mRNA expression in a sample include northern blotting and in situ hybridization (Parker & Barnes, Methods in Molecular Biology 106:247-283 (1999)); RNAse protection assays (Hod, Biotechniques 13:852-854 (1992)); and reverse transcription polymerase chain reaction (RT-PCR) (Weis et al., Trends in Genetics 8:263-264 (1992)). Alternatively, antibodies may be employed that can recognize specific duplexes, including DNA duplexes, RNA duplexes, and DNA-RNA hybrid duplexes or DNA-protein duplexes. Representative methods for sequencing-based gene expression analysis include Serial Analysis of Gene Expression (SAGE), and gene expression analysis by massively parallel signature sequencing (MPSS).

[0105] 2. Reverse Transcriptase PCR (RT-PCR)

[0106] Of the techniques listed above, the most sensitive and most flexible quantitative method is RT-PCR, which can be used to compare mRNA levels in different sample populations, in normal and tumor tissues, with or without drug treatment, to characterize patterns of gene expression, to discriminate between closely related mRNAs, and to analyze RNA structure.

[0107] The first step is the isolation of mRNA from a target sample. The starting material is typically total RNA isolated from human tumors or tumor cell lines, and corresponding normal tissues or cell lines, respectively. Thus RNA can be isolated from a variety of primary tumors, including breast, lung, colon, prostate, brain, liver, kidney, pancreas, spleen, thymus, testis, ovary, uterus, etc., tumor, or tumor cell lines, with pooled DNA from healthy donors. If the source of mRNA is a primary tumor, mRNA can be extracted, for example, from frozen or archived paraffin-embedded and fixed (e.g. formalin-fixed) tissue samples.

[0108] General methods for mRNA extraction are well known in the art and are disclosed in standard textbooks of molecular biology, including Ausubel et al., Current Protocols of Molecular Biology, John Wiley and Sons (1997). Methods for RNA extraction from paraffin embedded tissues are disclosed, for example, in Rupp and Locker, Lab Invest. 56:A67 (1987), and De Andrés et al., BioTechniques 18:42044 (1995). In particular, RNA isolation can be performed using purification kit, buffer set and protease from commercial manufacturers, such as Qiagen, according to the manufacturer's instructions. For example, total RNA from cells in culture can be isolated using Qiagen RNeasy mini-columns. Other commercially available RNA isolation kits include MasterPure™ Complete DNA and RNA Purification Kit (EPICENTRE®, Madison, Wis.), and Paraffin Block RNA Isolation Kit (Ambion, Inc.). Total RNA from tissue samples can be isolated using RNA Stat-60 (Tel-Test). RNA prepared from tumor can be isolated, for example, by cesium chloride density gradient centrifugation.

[0109] As RNA cannot serve as a template for PCR, the first step in gene expression profiling by RT-PCR is the reverse transcription of the RNA template into cDNA, followed by its exponential amplification in a PCR reaction. The two most commonly used reverse transcriptases are avilo myeloblastosis virus reverse transcriptase (AMV-RT) and Moloney murine leukemia virus reverse transcriptase (MMLV-RT). The reverse transcription step is typically primed using specific primers, random hexamers, or oligo-dT primers, depending on the circumstances and the goal of expression profiling. For example, extracted RNA can be reverse-transcribed using a GeneAmp RNA PCR kit (Perkin Elmer, Calif., USA), following the manufacturer's instructions. The derived cDNA can then be used as a template in the subsequent PCR reaction.

[0110] Although the PCR step can use a variety of thermostable DNA-dependent DNA polymerases, it typically employs the Taq DNA polymerase, which has a 5′-3′ nuclease activity but lacks a 3′-5′ proofreading endonuclease activity. Thus, TaqMan® PCR typically utilizes the 5′-nuclease activity of Taq or Tth polymerase to hydrolyze a hybridization probe bound to its target amplicon, but any enzyme with equivalent 5′ nuclease activity can be used. Two oligonucleotide primers are used to generate an amplicon typical of a PCR reaction. A third oligonucleotide, or probe, is designed to detect nucleotide sequence located between the two PCR primers. The probe is non-extendible by Taq DNA polymerase enzyme, and is labeled with a reporter fluorescent dye and a quencher fluorescent dye. Any laser-induced emission from the reporter dye is quenched by the quenching dye when the two dyes are located close together as they are on the probe. During the amplification reaction, the Taq DNA polymerase enzyme cleaves the probe in a template-dependent manner. The resultant probe fragments disassociate in solution, and signal from the released reporter dye is free from the quenching effect of the second fluorophore. One molecule of reporter dye is liberated for each new molecule synthesized, and detection of the unquenched reporter dye provides the basis for quantitative interpretation of the data.

[0111] TaqMan® RT-PCR can be performed using commercially available equipment, such as, for example, ABI PRISM 7700™ Sequence Detection System™ (Perkin-Elmer-Applied Biosystems, Foster City, Calif., USA), or Lightcycler (Roche Molecular Biochemicals, Mannheim, Germany). In a preferred embodiment, the 5′ nuclease procedure is run on a real-time quantitative PCR device such as the ABI PRISM 7700™ Sequence Detection System. The system consists of a thermocycler, laser, charge-coupled device (CCD), camera and computer. The system amplifies samples in a 96-well format on a thermocycler. During amplification, laser-induced fluorescent signal is collected in real-time through fiber optics cables for all 96 wells, and detected at the CCD. The system includes software for running the instrument and for analyzing the data.

[0112] 5′-Nuclease assay data are initially expressed as C_(t), or the threshold cycle. As discussed above, fluorescence values are recorded during every cycle and represent the amount of product amplified to that point in the amplification reaction. The point when the fluorescent signal is first recorded as statistically significant is the threshold cycle (C_(t)).

[0113] To minimize errors and the effect of sample-to-sample variation, RT-PCR is usually performed using an internal standard. The ideal internal standard is expressed at a constant level among different tissues, and is unaffected by the experimental treatment. RNAs most frequently used to normalize patterns of gene expression are mRNAs for the housekeeping genes glyceraldehyde-3-phosphate-dehydrogenase (GAPDH) and P-actin.

[0114] A more recent variation of the RT-PCR technique is the real time quantitative PCR, which measures PCR product accumulation through a dual-labeled fluorigenic probe (i.e., TaqMan® probe). Real time PCR is compatible both with quantitative competitive PCR, where internal competitor for each target sequence is used for normalization, and with quantitative comparative PCR using a normalization gene contained within the sample, or a housekeeping gene for RT-PCR. For further details see, e.g. Held et al., Genome Research 6:986-994 (1996).

[0115] The steps of a representative protocol for profiling gene expression using fixed, paraffin-embedded tissues as the RNA source, including mRNA isolation, purification, primer extension and amplification are given in various published journal articles {for example: T. E. Godfrey et al, J. Molec. Diagnostics 2: 84-91 [2000]; K. Specht et al., Am. J. Pathol. 158: 419-29 [2001]}. Briefly, a representative process starts with cutting about 10 μm thick sections of paraffin-embedded tumor tissue samples. The RNA is then extracted, and protein and DNA are removed. After analysis of the RNA concentration, RNA repair and/or amplification steps may be included, if necessary, and RNA is reverse transcribed using gene specific promoters followed by RT-PCR.

[0116] According to one aspect of the present invention, PCR primers and probes are designed based upon intron sequences present in the gene to be amplified. In this embodiment, the first step in the primer/probe design is the delineation of intron sequences within the genes. This can be done by publicly available software, such as the DNA BLAT software developed by Kent, W. J., Genome Res. 12(4):656-64 (2002), or by the BLAST software including its variations. Subsequent steps follow well established methods of PCR primer and probe design.

[0117] In order to avoid non-specific signals, it is important to mask repetitive sequences within the introns when designing the primers and probes. This can be easily accomplished by using the Repeat Masker program available on-line through the Baylor College of Medicine, which screens DNA sequences against a library of repetitive elements and returns a query sequence in which the repetitive elements are masked. The masked intron sequences can then be used to design primer and probe sequences using any commercially or otherwise publicly available primer/probe design packages, such as Primer Express (Applied Biosystems); MGB assay-by-design (Applied Biosystems); Primer3 (Steve Rozen and Helen J. Skaletsky (2000) Primer3 on the WWW for general users and for biologist programmers. In: Krawetz S, Misener S (eds) Bioinformatics Methods and Protocols: Methods in Molecular Biology. Humana Press, Totowa, N.J., pp 365-386)

[0118] The most important factors considered in PCR primer design include primer length, melting temperature (Tm), and G/C content, specificity, complementary primer sequences, and 3′-end sequence. In general, optimal PCR primers are generally 17-30 bases in length, and contain about 20-80%, such as, for example, about 50-60% G+C bases. Tm's between 50 and 80° C., e.g. about 50 to 70° C. are typically preferred.

[0119] For further guidelines for PCR primer and probe design see, e.g. Dieffenbach, C. W. et al., “General Concepts for PCR Primer Design” in: PCR Primer, A Laboratory Manual, Cold Spring Harbor Laboratory Press, New York, 1995, pp. 133-155; Innis and Gelfand, “Optimization of PCRs” in: PCR Protocols, A Guide to Methods and Applications, CRC Press, London, 1994, pp. 5-11; and Plasterer, T. N. Primerselect: Primer and probe design. Methods Mol. Biol. 70:520-527 (1997), the entire disclosures of which are hereby expressly incorporated by reference.

[0120] 3. Microarrays

[0121] Differential gene expression can also be identified, or confirmed using the microarray technique. Thus, the expression profile of breast cancer-associated genes can be measured in either fresh or paraffin-embedded tumor tissue, using microarray technology. In this method, polynucleotide sequences of interest (including cDNAs and oligonucleotides) are plated, or arrayed, on a microchip substrate. The arrayed sequences are then hybridized with specific DNA probes from cells or tissues of interest. Just as in the RT-PCR method, the source of mRNA typically is total RNA isolated from human tumors or tumor cell lines, and corresponding normal tissues or cell lines. Thus RNA can be isolated from a variety of primary tumors or tumor cell lines. If the source of mRNA is a primary tumor, mRNA can be extracted, for example, from frozen or archived paraffin-embedded and fixed (e.g. formalin-fixed) tissue samples, which are routinely prepared and preserved in everyday clinical practice.

[0122] In a specific embodiment of the microarray technique, PCR amplified inserts of cDNA clones are applied to a substrate in a dense array. Preferably at least 10,000 nucleotide sequences are applied to the substrate. The microarrayed genes, immobilized on the microchip at 10,000 elements each, are suitable for hybridization under stringent conditions. Fluorescently labeled cDNA probes may be generated through incorporation of fluorescent nucleotides by reverse transcription of RNA extracted from tissues of interest. Labeled cDNA probes applied to the chip hybridize with specificity to each spot of DNA on the array. After stringent washing to remove non-specifically bound probes, the chip is scanned by confocal laser microscopy or by another detection method, such as a CCD camera. Quantitation of hybridization of each arrayed element allows for assessment of corresponding mRNA abundance. With dual color fluorescence, separately labeled cDNA probes generated from two sources of RNA are hybridized pairwise to the array. The relative abundance of the transcripts from the two sources corresponding to each specified gene is thus determined simultaneously. The miniaturized scale of the hybridization affords a convenient and rapid evaluation of the expression pattern for large numbers of genes. Such methods have been shown to have the sensitivity required to detect rare transcripts, which are expressed at a few copies per cell, and to reproducibly detect at least approximately two-fold differences in the expression levels (Schena et al., Proc. Natl. Acad. Sci. USA 93(2):106-149 (1996)). Microarray analysis can be performed by commercially available equipment, following manufacturer's protocols, such as by using the Affymetrix GenChip technology, or Incyte's microarray technology.

[0123] The development of microarray methods for large-scale analysis of gene expression makes it possible to search systematically for molecular markers of cancer classification and outcome prediction in a variety of tumor types.

[0124] 4. Serial Analysis of Gene Expression (SAGE)

[0125] Serial analysis of gene expression (SAGE) is a method that allows the simultaneous and quantitative analysis of a large number of gene transcripts, without the need of providing an individual hybridization probe for each transcript. First, a short sequence tag (about 10-14 bp) is generated that contains sufficient information to uniquely identify a transcript, provided that the tag is obtained from a unique position within each transcript. Then, many transcripts are linked together to form long serial molecules, that can be sequenced, revealing the identity of the multiple tags simultaneously. The expression pattern of any population of transcripts can be quantitatively evaluated by determining the abundance of individual tags, and identifying the gene corresponding to each tag. For more details see, e.g. Velculescu et al., Science 270:484-487 (1995); and Velculescu et al., Cell 88:243-51 (1997).

[0126] 5. MassARRA Y Technology

[0127] The MassARRAY (Sequenom, San Diego, Calif.) technology is an automated, high-throughput method of gene expression analysis using mass spectrometry (MS) for detection. According to this method, following the isolation of RNA, reverse transcription and PCR amplification, the cDNAs are subjected to primer extension. The cDNA-derived primer extension products are purified, and dipensed on a chip array that is pre-loaded with the components needed for MALTI-TOF MS sample preparation. The various cDNAs present in the reaction are quantitated by analyzing the peak areas in the mass spectrum obtained.

[0128] 6. Gene Expression Analysis by Massively Parallel Signature Sequencing (MPSS)

[0129] This method, described by Brenner et al., Nature Biotechnology 18:630-634 (2000), is a sequencing approach that combines non-gel-based signature sequencing with in vitro cloning of millions of templates on separate 5 μm diameter microbeads. First, a microbead library of DNA templates is constructed by in vitro cloning. This is followed by the assembly of a planar array of the template-containing microbeads in a flow cell at a high density (typically greater than 3×10⁶ microbeads/cm²). The free ends of the cloned templates on each microbead are analyzed simultaneously, using a fluorescence-based signature sequencing method that does not require DNA fragment separation. This method has been shown to simultaneously and accurately provide, in a single operation, hundreds of thousands of gene signature sequences from a yeast cDNA library.

[0130] 7. Immunohistochemistry

[0131] Immunohistochemistry methods are also suitable for detecting the expression levels of the prognostic markers of the present invention. Thus, antibodies or antisera, preferably polyclonal antisera, and most preferably monoclonal antibodies specific for each marker are used to detect expression. The antibodies can be detected by direct labeling of the antibodies themselves, for example, with radioactive labels, fluorescent labels, hapten labels such as, biotin, or an enzyme such as horse radish peroxidase or alkaline phosphatase. Alternatively, unlabeled primary antibody is used in conjunction with a labeled secondary antibody, comprising antisera, polyclonal antisera or a monoclonal antibody specific for the primary antibody. Immunohistochemistry protocols and kits are well known in the art and are commercially available.

[0132] 8. Proteomics

[0133] The term “proteome” is defined as the totality of the proteins present in a sample (e.g. tissue, organism, or cell culture) at a certain point of time. Proteomics includes, among other things, study of the global changes of protein expression in a sample (also referred to as “expression proteomics”). Proteomics typically includes the following steps: (1) separation of individual proteins in a sample by 2-D gel electrophoresis (2-D PAGE); (2) identification of the individual proteins recovered from the gel, e.g. my mass spectrometry or N-terminal sequencing, and (3) analysis of the data using bioinformatics. Proteomics methods are valuable supplements to other methods of gene expression profiling, and can be used, alone or in combination with other methods, to detect the products of the prognostic markers of the present invention.

[0134] 9. General Description of the mRNA Isolation, Purification and Amplification

[0135] The steps of a representative protocol for profiling gene expression using fixed, paraffin-embedded tissues as the RNA source, including mRNA isolation, purification, primer extension and amplification are given in various published journal articles {for example: T. E. Godfrey et al. J. Molec. Diagnostics 2: 84-91 [2000]; K. specht et al., Am. J. Pathol. 158: 419-29 [2001]}. Briefly, a representative process starts with cutting about 10 μm thick sections of paraffin-embedded tumor tissue samples. The RNA is then extracted, and protein and DNA are removed. After analysis of the RNA concentration, RNA repair and/or amplification steps may be included, if necessary, and RNA is reverse transcribed using gene specific promoters followed by RT-PCR. Finally, the data are analyzed to identify the best treatment option(s) available to the patient on the basis of the characteristic gene expression pattern identified in the tumor sample examined.

[0136] 10. Breast Cancer Gene Set, Assayed Gene Subsequences, and Clinical Application of Gene Expression Data

[0137] An important aspect of the present invention is to use the measured expression of certain genes by breast cancer tissue to provide prognostic information. For this purpose it is necessary to correct for (normalize away) both differences in the amount of RNA assayed and variability in the quality of the RNA used. Therefore, the assay typically measures and incorporates the expression of certain normalizing genes, including well known housekeeping genes, such as GAPDH and Cyp1. Alternatively, normalization can be based on the mean or median signal (Ct) of all of the assayed genes or a large subset thereof (global normalization approach). On a gene-by-gene basis, measured normalized amount of a patient tumor mRNA is compared to the amount found in a breast cancer tissue reference set. The number (N) of breast cancer tissues in this reference set should be sufficiently high to ensure that different reference sets (as a whole) behave essentially the same way. If this condition is met, the identity of the individual breast cancer tissues present in a particular set will have no significant impact on the relative amounts of the genes assayed. Usually, the breast cancer tissue reference set consists of at least about 30, preferably at least about 40 different FPE breast cancer tissue specimens. Unless noted otherwise, normalized expression levels for each mRNA/tested tumor/patient will be expressed as a percentage of the expression level measured in the reference set. More specifically, the reference set of a sufficiently high number (e.g. 40) of tumors yields a distribution of normalized levels of each mRNA species. The level measured in a particular tumor sample to be analyzed falls at some percentile within this range, which can be determined by methods well known in the art. Below, unless noted otherwise, reference to expression levels of a gene assume normalized expression relative to the reference set although this is not always explicitly stated.

[0138] Further details of the invention will be described in the following non-limiting Example

EXAMPLE

[0139] A Phase II Study of Gene Expression in 79 Malignant Breast Tumors

[0140] A gene expression study was designed and conducted with the primary goal to molecularly characterize gene expression in paraffin-embedded, fixed tissue samples of invasive breast ductal carcinoma, and to explore the correlation between such molecular profiles and disease-free survival.

[0141] Study Design

[0142] Molecular assays were performed on paraffin-embedded, formalin-fixed primary breast tumor tissues obtained from 79 individual patients diagnosed with invasive breast cancer. All patients in the study had 10 or more positive nodes. Mean age was 57 years, and mean clinical tumor size was 4.4 cm. Patients were included in the study only if histopathologic assessment, performed as described in the Materials and Methods section, indicated adequate amounts of tumor tissue and homogeneous pathology.

[0143] Materials and Methods

[0144] Each representative tumor block was characterized by standard histopathology for diagnosis, semi-quantitative assessment of amount of tumor, and tumor grade. A total of 6 sections (10 microns in thickness each) were prepared and placed in two Costar Brand Microcentrifuge Tubes (Polypropylene, 1.7 mL tubes, clear; 3 sections in each tube). If the tumor constituted less than 30% of the total specimen area, the sample may have been crudely dissected by the pathologist, using gross microdissection, putting the tumor tissue directly into the Costar tube.

[0145] If more than one tumor block was obtained as part of the surgical procedure, the block most representative of the pathology was used for analysis.

[0146] Gene Expression Analysis

[0147] mRNA was extracted and purified from fixed, paraffin-embedded tissue samples, and prepared for gene expression analysis as described in section 9 above.

[0148] Molecular assays of quantitative gene expression were performed by RT-PCR, using the ABI PRISM 7900™ Sequence Detection System™ (Perkin-Elmer-Applied Biosystems, Foster City, Calif., USA). ABI PRISM 7900™ consists of a thermocycler, laser, charge-coupled device (CCD), camera and computer. The system amplifies samples in a 384-well format on a thermocycler. During amplification, laser-induced fluorescent signal is collected in real-time through fiber optics cables for all 384 wells, and detected at the CCD. The system includes software for running the instrument and for analyzing the data.

[0149] Analysis and Results

[0150] Tumor tissue was analyzed for 185 cancer-related genes and 7 reference genes. The threshold cycle (CT) values for each patient were normalized based on the median of the 7 reference genes for that particular patient. Clinical outcome data were available for all patients from a review of registry data and selected patient charts.

[0151] Outcomes were classified as:

[0152] 0 died due to breast cancer or to unknown cause or alive with breast cancer recurrence;

[0153] 1 alive without breast cancer recurrence or died due to a cause other than breast cancer

[0154] Analysis was performed by:

[0155] 1. Analysis of the relationship between normalized gene expression and the binary outcomes of 0 or 1.

[0156] 2. Analysis of the relationship between normalized gene expression and the time to outcome (0 or 1 as defined above) where patients who were alive without breast cancer recurrence or who died due to a cause other than breast cancer were censored. This approach was used to evaluate the prognostic impact of individual genes and also sets of multiple genes.

[0157] Analysis of Patients with Invasive Breast Carcinoma by Binary Approach

[0158] In the first (binary) approach, analysis was performed on all 79 patients with invasive breast carcinoma. A t test was performed on the groups of patients classified as either no recurrence and no breast cancer related death at three years, versus recurrence, or breast cancer-related death at three years, and the p-values for the differences between the groups for each gene were calculated.

[0159] Table 1 lists the 47 genes for which the p-value for the differences between the groups was <0.10. The first column of mean expression values pertains to patients who neither had a metastatic recurrence of nor died from breast cancer. The second column of mean expression values pertains to patients who either had a metastatic recurrence of or died from breast cancer. TABLE 1 Mean Mean t-value df p Valid N Valid N Bcl2 −0.15748 −1.22816 4.00034 75 0.000147 35 42 PR −2.67225 −5.49747 3.61540 75 0.000541 35 42 IGF1R −0.59390 −1.71506 3.49158 75 0.000808 35 42 BAG1 0.18844 −0.68509 3.42973 75 0.000985 35 42 CD68 −0.52275 0.10983 −3.41186 75 0.001043 35 42 EstR1 −0.35581 −3.00699 3.32190 75 0.001384 35 42 CTSL −0.64894 −0.09204 −3.26781 75 0.001637 35 42 IGFBP2 −0.81181 −1.78398 3.24158 75 0.001774 35 42 GATA3 1.80525 0.57428 3.15608 75 0.002303 35 42 TP53BP2 −4.71118 −6.09289 3.02888 75 0.003365 35 42 EstR1 3.67801 1.64693 3.01073 75 0.003550 35 42 CEGP1 −2.02566 −4.25537 2.85620 75 0.005544 35 42 SURV −3.67493 −2.96982 −2.70544 75 0.008439 35 42 p27 0.80789 0.28807 2.55401 75 0.012678 35 42 Chk1 −3.37981 −2.80389 −2.46979 75 0.015793 35 42 BBC3 −4.71789 −5.62957 2.46019 75 0.016189 35 42 ZNF217 1.10038 0.62730 2.42282 75 0.017814 35 42 EGFR −2.88172 −2.20556 −2.34774 75 0.021527 35 42 CD9 1.29955 0.91025 2.31439 75 0.023386 35 42 MYBL2 −3.77489 −3.02193 −2.29042 75 0.024809 35 42 HIF1A −0.44248 0.03740 −2.25950 75 0.026757 35 42 GRB7 −1.96063 −1.05007 −2.25801 75 0.026854 35 42 pS2 −1.00691 −3.13749 2.24070 75 0.028006 35 42 RIZ1 −7.62149 −8.38750 2.20226 75 0.030720 35 42 ErbB3 −6.89508 −7.44326 2.16127 75 0.033866 35 42 TOP2B 0.45122 0.12665 2.14616 75 0.035095 35 42 MDM2 1.09049 0.69001 2.10967 75 0.038223 35 42 PRAME −6.40074 −7.70424 2.08126 75 0.040823 35 42 GUS −1.51683 −1.89280 2.05200 75 0.043661 35 42 RAD51C −5.85618 −6.71334 2.04575 75 0.044288 35 42 AIB1 −3.08217 −2.28784 −2.00600 75 0.048462 35 42 STK15 −3.11307 −2.59454 −2.00321 75 0.048768 35 42 GAPDH −0.35829 −0.02292 −1.94326 75 0.055737 35 42 FHIT −3.00431 −3.67175 1.86927 75 0.065489 35 42 KRT19 2.52397 2.01694 1.85741 75 0.067179 35 42 TS −2.83607 −2.29048 −1.83712 75 0.070153 35 42 GSTM1 −3.69140 −4.38623 1.83397 75 0.070625 35 42 G- 0.31875 −0.15524 1.80823 75 0.074580 35 42 Catenin AKT2 0.78858 0.46703 1.79276 75 0.077043 35 42 CCNB1 −4.26197 −3.51628 −1.78803 75 0.077810 35 42 PI3KC2A −2.27401 −2.70265 1.76748 75 0.081215 35 42 FBXO5 −4.72107 −4.24411 −1.75935 75 0.082596 35 42 DR5 −5.80850 −6.55501 1.74345 75 0.085353 35 42 CIAP1 −2.81825 −3.09921 1.72480 75 0.088683 35 42 MCM2 −2.87541 −2.50683 −1.72061 75 0.089445 35 42 CCND1 1.30995 0.80905 1.68794 75 0.095578 35 42 EIF4E −5.37657 −6.47156 1.68169 75 0.096788 35 42

[0160] In the foregoing Table 1, negative t-values indicate higher expression, associated with worse outcomes, and, inversely, higher (positive) t-values indicate higher expression associated with better outcomes. Thus, for example, elevated expression of the CD68 gene (t-value=−3.41, CT mean alive<CT mean deceased) indicates a reduced likelihood of disease free survival. Similarly, elevated expression of the BC12 gene (t-value=4.00; CT mean alive>CT mean deceased) indicates an increased likelihood of disease free survival.

[0161] Based on the data set forth in Table 1, the expression of any of the following genes in breast cancer above a defined expression threshold indicates a reduced likelihood of survival without cancer recurrence following surgery: Grb7, CD68, CTSL, Chk1, Her2, STK15, AIB1, SURV, EGFR, MYBL2, HIF1α.

[0162] Based on the data set forth in Table 1, the expression of any of the following genes in breast cancer above a defined expression threshold indicates a better prognosis for survival without cancer recurrence following surgery: TP53BP2, PR, Bc12, KRT14, EstR1, IGFBP2, BAG1, CEGP1, KLK10, β Catenin, GSTM1, FHIT, Riz1, IGF1, BBC3, IGFR1, TBP, p27, IRS1, IGF1R, GATA3, CEGP1, ZNF217, CD9, pS2, ErbB3, TOP2B, MDM2, RAD51, and KRT19.

[0163] Analysis of ER Positive Patients by Binary Approach

[0164] 57 patients with normalized CT for estrogen receptor (ER)>0 (i.e., ER positive patients) were subjected to separate analysis. A t test was performed on the two groups of patients classified as either no recurrence and no breast cancer related death at three years, or recurrence or breast cancer-related death at three years, and the p-values for the differences between the groups for each gene were calculated. Table 2, below, lists the genes where the p-value for the differences between the groups was <0.105. The first column of mean expression values pertains to patients who neither had a metastatic recurrence nor died from breast cancer. The second column of mean expression values pertains to patients who either had a metastatic recurrence of or died from breast cancer. TABLE 2 Mean Mean t-value df p Valid N Valid N IGF1R −0.13975 −1.00435 3.65063 55 0.000584 30 27 Bcl2 0.15345 −0.70480 3.55488 55 0.000786 30 27 CD68 −0.54779 0.19427 −3.41818 55 0.001193 30 27 HNF3A 0.39617 −0.63802 3.20750 55 0.002233 30 27 CTSL −0.66726 0.00354 −3.20692 55 0.002237 30 27 TP53BP2 −4.81858 −6.44425 3.13698 55 0.002741 30 27 GATA3 2.33386 1.40803 3.02958 55 0.003727 30 27 BBC3 −4.54979 −5.72333 2.91943 55 0.005074 30 27 RAD51C −5.63363 −6.94841 2.85475 55 0.006063 30 27 BAG1 0.31087 −0.50669 2.61524 55 0.011485 30 27 IGFBP2 −0.49300 −1.30983 2.59121 55 0.012222 30 27 FBXO5 −4.86333 −4.05564 −2.56325 55 0.013135 30 27 EstR1 0.68368 −0.66555 2.56090 55 0.013214 30 27 PR −1.89094 −3.86602 2.52803 55 0.014372 30 27 SURV −3.87857 −3.10970 −2.49622 55 0.015579 30 27 CD9 1.41691 0.91725 2.43043 55 0.018370 30 27 RB1 −2.51662 −2.97419 2.41221 55 0.019219 30 27 EPHX1 −3.91703 −5.85097 2.29491 55 0.025578 30 27 CEGP1 −1.18600 −2.95139 2.26608 55 0.027403 30 27 CCNB1 −4.44522 −3.35763 −2.25148 55 0.028370 30 27 TRAIL 0.34893 −0.56574 2.20372 55 0.031749 30 27 EstR1 4.60346 3.60340 2.20223 55 0.031860 30 27 DR5 −5.71827 −6.79088 2.14548 55 0.036345 30 27 MCM2 −2.96800 −2.48458 −2.10518 55 0.039857 30 27 Chk1 −3.46968 −2.85708 −2.08597 55 0.041633 30 27 p27 0.94714 0.49656 2.04313 55 0.045843 30 27 MYBL2 −3.97810 −3.14837 −2.02921 55 0.047288 30 27 GUS −1.42486 −1.82900 1.99758 55 0.050718 30 27 P53 −1.08810 −1.47193 1.92087 55 0.059938 30 27 HIF1A −0.40925 0.11688 −1.91278 55 0.060989 30 27 cMet −6.36835 −5.58479 −1.88318 55 0.064969 30 27 EGFR −2.95785 −2.28105 −1.86840 55 0.067036 30 27 MTA1 −7.55365 −8.13656 1.81479 55 0.075011 30 27 RIZ1 −7.52785 −8.25903 1.79518 55 0.078119 30 27 ErbB3 −6.62488 −7.10826 1.79255 55 0.078545 30 27 TOP2B 0.54974 0.27531 1.74888 55 0.085891 30 27 EIF4E −5.06603 −6.31426 1.68030 55 0.098571 30 27 TS −2.95042 −2.36167 −1.67324 55 0.099959 30 27 STK15 −3.25010 −2.72118 −1.64822 55 0.105010 30 27

[0165] For each gene, a classification algorithm was utilized to identify the best threshold value (CT) for using each gene alone in predicting clinical outcome.

[0166] Based on the data set forth in Table 2, expression of the following genes in ER-positive cancer above a defined expression level is indicative of a reduced likelihood of survival without cancer recurrence following surgery: CD68; CTSL; FBXO5; SURV; CCNB1; MCM2; Chk1; MYBL2; HIF1A; cMET; EGFR; TS; STK15. Many of these genes (CD68, CTSL, SURV, CCNB1, MCM2, Chk1, MYBL2, EGFR, and STK15) were also identified as indicators of poor prognosis in the previous analysis, not limited to ER-positive breast cancer. Based on the data set forth in Table 2, expression of the following genes in ER-positive cancer above a defined expression level is indicative of a better prognosis for survival without cancer recurrence following surgery: IGFR1; BC12; HNF3A; TP53BP2; GATA3; BBC3; RAD51C; BAG1; IGFBP2; PR; CD9; RB1; EPHX1; CEGP1; TRAIL; DR5; p27; p53; MTA; RIZ1; ErbB3; TOP2B; EIF4E. Of the latter genes, IGFR1; BC12; TP53BP2; GATA3; BBC3; RAD51C; BAG1; IGFBP2; PR; CD9; CEGP1; DR5; p27; RIZ1; ErbB3; TOP2B; EIF4E have also been identified as indicators of good prognosis in the previous analysis, not limited to ER-positive breast cancer.

[0167] Analysis of ER Negative Patients by Binary Approach

[0168] Twenty patients with normalized CT for estrogen receptor (ER)<1.6 (i.e., ER negative patients) were subjected to separate analysis. A t test was performed on the two groups of patients classified as either no recurrence and no breast cancer related death at three years, or recurrence or breast cancer-related death at three years, and the p-values for the differences between the groups for each gene were calculated. Table 3 lists the genes where the p-value for the differences between the groups was <0.118. The first column of mean expression values pertains to patients who neither had a metastatic recurrence nor died from breast cancer. The second column of mean expression values pertains to patients who either had a metastatic recurrence of or died from breast cancer. TABLE 3 Mean Mean t-value df p Valid N Valid N KRT14 −1.95323 −6.69231 4.03303 18 0.000780 5 15 KLK10 −2.68043 −7.11288 3.10321 18 0.006136 5 15 CCND1 −1.02285 0.03732 −2.77992 18 0.012357 5 15 Upa −0.91272 −0.04773 −2.49460 18 0.022560 5 15 HNF3A −6.04780 −2.36469 −2.43148 18 0.025707 5 15 Maspin −3.56145 −6.18678 2.40169 18 0.027332 5 15 CDH1 −3.54450 −2.34984 −2.38755 18 0.028136 5 15 HER2 −1.48973 1.53108 −2.35826 18 0.029873 5 15 GRB7 −2.55289 0.00036 −2.32890 18 0.031714 5 15 AKT1 −0.36849 0.46222 −2.29737 18 0.033807 5 15 TGFA −4.03137 −5.67225 2.28546 18 0.034632 5 15 FRP1 1.45776 −1.39459 2.27884 18 0.035097 5 15 STMY3 −1.59610 −0.26305 −2.23191 18 0.038570 5 15 Contig −4.27585 −7.34338 2.18700 18 0.042187 5 15 27882 A-Catenin −1.19790 −0.39085 −2.15624 18 0.044840 5 15 VDR −4.37823 −2.37167 −2.15620 18 0.044844 5 15 GRO1 −3.65034 −5.97002 2.12286 18 0.047893 5 15 MCM3 −3.86041 −5.55078 2.10030 18 0.050061 5 15 B-actin 4.69672 5.19190 −2.04951 18 0.055273 5 15 HIF1A −0.64183 −0.10566 −2.02301 18 0.058183 5 15 MMP9 −8.90613 −7.35163 −1.88747 18 0.075329 5 15 VEGF 0.37904 1.10778 −1.87451 18 0.077183 5 15 PRAME −4.95855 −7.41973 1.86668 18 0.078322 5 15 AIB1 −3.12245 −1.92934 −1.86324 18 0.078829 5 15 KRT5 −1.32418 −3.62027 1.85919 18 0.079428 5 15 KRT18 1.08383 2.25369 −1.83831 18 0.082577 5 15 KRT17 −0.69073 −3.56536 1.78449 18 0.091209 5 15 P14ARF −1.87104 −3.36534 1.63923 18 0.118525 5 15

[0169] Based on the data set forth in Table 3, expression of the following genes in ER-negative cancer above a defined expression level is indicative of a reduced likelihood of survival without cancer recurrence (p<0.05): CCND1; UPA; HNF3A; CDH1; Her2; GRB7; AKT1; STMY3; α-Catenin; VDR; GRO1. Only 2 of these genes (Her2 and Grb7) were also identified as indicators of poor prognosis in the previous analysis, not limited to ER-negative breast cancer. Based on the data set forth in Table 3, expression of the following genes in ER-negative cancer above a defined expression level is indicative of a better prognosis for survival without cancer recurrence (KT14; KLK10; Maspin, TGFα, and FRP1. Of the latter genes, only KLK10 has been identified as an indicator of good prognosis in the previous analysis, not limited to ER-negative breast cancer.

[0170] Analysis of Multiple Genes and Indicators of Outcome

[0171] Two approaches were taken in order to determine whether using multiple genes would provide better discrimination between outcomes.

[0172] First, a discrimination analysis was performed using a forward stepwise approach. Models were generated that classified outcome with greater discrimination than was obtained with any single gene alone.

[0173] According to a second approach (time-to-event approach), for each gene a Cox Proportional Hazards model (see, e.g. Cox, D. R., and Oakes, D. (1984), ANALYSIS of Survival Data, Chapman and Hall, London, New York) was defined with time to recurrence or death as the dependent variable, and the expression level of the gene as the independent variable. The genes that have a p-value <0.10 in the Cox model were identified. For each gene, the Cox model provides the relative risk (RR) of recurrence or death for a unit change in the expression of the gene. One can choose to partition the patients into subgroups at any threshold value of the measured expression (on the CT scale), where all patients with expression values above the threshold have higher risk, and all patients with expression values below the threshold have lower risk, or vice versa, depending on whether the gene is an indicator of bad (RR>1.01) or good (RR<1.01) prognosis. Thus, any threshold value will define subgroups of patients with respectively increased or decreased risk. The results are summarized in Table 4. The third column, with the heading: exp(coef), shows RR values. TABLE 4 Gene coef exp(coef) se(coef) z p TP53BP2 −0.21892 0.803386 0.068279 −3.20625 0.00134 GRB7 0.235697 1.265791 0.073541 3.204992 0.00135 PR −0.10258 0.90251 0.035864 −2.86018 0.00423 CD68 0.465623 1.593006 0.167785 2.775115 0.00552 Bcl2 −0.26769 0.765146 0.100785 −2.65603 0.00791 KRT14 −0.11892 0.887877 0.046938 −2.53359 0.0113 PRAME −0.13707 0.871912 0.054904 −2.49649 0.0125 CTSL 0.431499 1.539564 0.185237 2.329444 0.0198 EstR1 −0.07686 0.926018 0.034848 −2.20561 0.0274 Chk1 0.284466 1.329053 0.130823 2.174441 0.0297 IGFBP2 −0.2152 0.806376 0.099324 −2.16669 0.0303 HER2 0.155303 1.168011 0.072633 2.13818 0.0325 BAG1 −0.22695 0.796959 0.106377 −2.13346 0.0329 CEGP1 −0.07879 0.924236 0.036959 −2.13177 0.033 STK15 0.27947 1.322428 0.132762 2.105039 0.0353 KLK10 −0.11028 0.895588 0.05245 −2.10248 0.0355 B.Catenin −0.16536 0.847586 0.084796 −1.95013 0.0512 EstR1 −0.0803 0.922842 0.042212 −1.90226 0.0571 GSTM1 −0.13209 0.876266 0.072211 −1.82915 0.0674 TOP2A −0.11148 0.894512 0.061855 −1.80222 0.0715 AlB1 0.152968 1.165288 0.086332 1.771861 0.0764 FHIT −0.15572 0.855802 0.088205 −1.7654 0.0775 RIZ1 −0.17467 0.839736 0.099464 −1.75609 0.0791 SURV 0.185784 1.204162 0.106625 1.742399 0.0814 IGF1 −0.10499 0.900338 0.060482 −1.73581 0.0826 BBC3 −0.1344 0.874243 0.077613 −1.73163 0.0833 IGF1R −0.13484 0.87358 0.077889 −1.73115 0.0834 DIABLO 0.284336 1.32888 0.166556 1.707148 0.0878 TBP −0.34404 0.7089 0.20564 −1.67303 0.0943 p27 −0.26002 0.771033 0.1564 −1.66256 0.0964 IRS1 −0.07585 0.926957 0.046096 −1.64542 0.0999

[0174] The binary and time-to-event analyses, with few exceptions, identified the same genes as prognostic markers. For example, comparison of Tables 1 and 4 shows that 10 genes were represented in the top 15 genes in both lists. Furthermore, when both analyses identified the same gene at [p<0.10], which happened for 21 genes, they were always concordant with respect to the direction (positive or negative sign) of the correlation with survival/recurrence. Overall, these results strengthen the conclusion that the identified markers have significant prognostic value.

[0175] For Cox models comprising more than two genes (multivariate models), stepwise entry of each individual gene into the model is performed, where the first gene entered is pre-selected from among those genes having significant univariate p-values, and the gene selected for entry into the model at each subsequent step is the gene that best improves the fit of the model to the data. This analysis can be performed with any total number of genes. In the analysis the results of which are shown below, stepwise entry was performed for up to 10 genes.

[0176] Multivariate analysis is performed using the following equation:

RR=exp[coef(geneA)×Ct(geneA)+coef(geneB)×Ct(geneB)+coef(geneC)×Ct(geneC)+ . . . ].

[0177] In this equation, coefficients for genes that are predictors of beneficial outcome are positive numbers and coefficients for genes that are predictors of unfavorable outcome are negative numbers. The “Ct” values in the equation are ACts, i.e. reflect the difference between the average normalized Ct value for a population and the normalized Ct measured for the patient in question. The convention used in the present analysis has been that ACts below and above the population average have positive signs and negative signs, respectively (reflecting greater or lesser mRNA abundance). The relative risk (RR) calculated by solving this equation will indicate if the patient has an enhanced or reduced chance of long-term survival without cancer recurrence.

[0178] Multivariate Gene Analysis of 79 Patients with Invasive Breast Carcinoma

[0179] A multivariate stepwise analysis, using the Cox Proportional Hazards Model, was performed on the gene expression data obtained for all 79 patients with invasive breast carcinoma. The following ten-gene sets have been identified by this analysis as having particularly strong predictive value of patient survival:

[0180] (a) TP53BP2, Bc12, BAD, EPHX1, PDGFRβ, DIABLO, XIAP, YB1, CA9, and KRT8.

[0181] (b) GRB7, CD68, TOP2A, Bc12, DIABLO, CD3, ID1, PPM1D, MCM6, and WISP1.

[0182] (c) PR, TP53BP2, PRAME, DIABLO, CTSL, IGFBP2, TIMP1, CA9, MMP9, and COX2.

[0183] (d) CD68, GRB7, TOP2A, Bc12, DIABLO, CD3, ID1, PPM1D, MCM6, and WISP1.

[0184] (e) Bc12, TP53BP2, BAD, EPHX1, PDGFRβ, DIABLO, XIAP, YB1, CA9, and KRT8.

[0185] (f) KRT14, KRT5, PRAME, TP53BP2, GUS1, AIB1, MCM3, CCNE1, MCM6, and ID1.

[0186] (g) PRAME, TP53BP2, EstR1, DIABLO, CTSL, PPM1D, GRB7, DAPK1, BBC3, and VEGFB.

[0187] (h) CTSL2, GRB7, TOP2A, CCNB1, Bc12, DIABLO, PRAME, EMS1, CA9, and EpCAM.

[0188] (i) EstR1, TP53BP2, PRAME, DIABLO, CTSL, PPM1D, GRB7, DAPK1, BBC3, and VEGFB.

[0189] (k) Chk1, PRAME, p53BP2, GRB7, CA9, CTSL, CCNB1, TOP2A, tumor size, and IGFBP2.

[0190] (l) IGFBP2, GRB7, PRAME, DIABLO, CTSL, β-Catenin, PPM1D, Chk1, WISP1, and LOT1.

[0191] (m) HER2, TP53BP2, Bc12, DIABLO, TIMP1, EPHX1, TOP2A, TRAIL, CA9, and AREG.

[0192] (n) BAG1, TP53BP2, PRAME, IL6, CCNB1, PAIL, AREG, tumor size, CA9, and Ki67.

[0193] (o) CEGP1, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, STK15, and AKT2, and FGF18.

[0194] (p) STK15, TP53BP2, PRAME, IL6, CCNE1, AKT2, DIABLO, cMet, CCNE2, and COX2.

[0195] (q) KLK10, EstR1, TP53BP2, PRAME, DIABLO, CTSL, PPM1D, GRB7, DAPK1, and BBC3.

[0196] (r) AIB1, TP53BP2, Bc12, DIABLO, TIMP1, CD3, p53, CA9, GRB7, and EPHX1

[0197] (s) BBC3, GRB7, CD68, PRAME, TOP2A, CCNB1, EPHX1, CTSL GSTM1, and APC.

[0198] (t) CD9, GRB7, CD68, TOP2A, Bc12, CCNB1, CD3, DIABLO, ID1, and PPM1D.

[0199] (w) EGFR, KRT14, GRB7, TOP2A, CCNB1, CTSL, Bc12, TP, KLK10, and CA9.

[0200] (x) HIF1α, PR, DIABLO, PRAME, Chk1, AKT2, GRB7, CCNE1, TOP2A, and CCNB1.

[0201] (y) MDM2, TP53BP2, DIABLO, Bc12, AIB1, TIMP1, CD3, p53, CA9, and HER2.

[0202] (z) MYBL2, TP53BP2, PRAME, IL6, Bc12, DIABLO, CCNE1, EPHX1, TIMP1, and CA9.

[0203] (aa) p27, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, STK15, AKT2, and ID1.

[0204] (ab) RAD51, GRB7, CD68, TOP2A, CIAP2, CCNB1, BAG1, IL6, FGFR1, and TP53BP2.

[0205] (ac) SURV, GRB7, TOP2A, PRAME, CTSL, GSTM1, CCNB1, VDR, CA9, and CCNE2.

[0206] (ad) TOP2B, TP53BP2, DIABLO, Bc12, TIMP1, AIB1, CA9, p53, KRT8, and BAD.

[0207] (ae) ZNF217, GRB7, p53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, APC4, and β-Catenin.

[0208] While the present invention has been described with reference to what are considered to be the specific embodiments, it is to be understood that the invention is not limited to such embodiments. To the contrary, the invention is intended to cover various modifications and equivalents included within the spirit and scope of the appended claims. For example, while the disclosure focuses on the identification of various breast cancer associated genes and gene sets, and on the personalized prognosis of breast cancer, similar genes, gene sets and methods concerning other types of cancer are specifically within the scope herein.

[0209] All references cited throughout the disclosure are hereby expressly incorporated by reference. TABLE 5A Gene Accession Seq AIB1 NM_006534 GCGGCGAGTTTCCGATTTAAAGCTGAGCTGCGAGGAAAATGGCGGCGGGAGGATCAAAATACTTGCTGGATGGTGGACTCA AKT1 NM_005163 CGCTTCTATGGCGCTGAGATTGTGTCAGCCCTGGACTACCTGCACTCGGAGAAGAACGTGGTGTACCGGGA AKT2 NM_001626 TCCTGCCACCCTTCAAACCTCAGGTCACGTCCGAGGTCGACACAAGGTACTTCGATGATGAATTTACCGCC APC NM_000038 GGACAGCAGGAATGTGTTTCTCCATACAGGTCACGGGGAGCCAATGGTTCAGAAACAAATCGAGTGGGT AREG NM_001657 TGTGAGTGAAATGCCTTCTAGTAGTGAACCGTCCTCGGGAGCCGACTATGACTACTCAGAAGAGTATGATAACGAACCACAA B-actin NM_001101 CAGCAGATGTGGATCAGCAAGCAGGAGTATGACGAGTCCGGCCCCTCCATCGTCCACCGCAAATGC B-Catenin NM_001904 GGCTCTTGTGCGTACTGTCCTTCGGGCTGGTGACAGGGAAGACATCACTGAGCCTGCCATCTGTGCTCTTCGTCATCTGA BAD NM_032989 GGGTCAGGTGCCTCGAGATCGGGCTTGGGCCCAGAGCATGTTCCAGATCCCAGAGTTTGAGCCGAGTGAGCAG BAG1 NM_004323 CGTTGTCAGCACTTGGAATACAAGATGGTTGCCGGGTCATGTTAATTGGGAAAAAGAACAGTCCACAGGAAGAGGTTGAAC BBC3 NM_014417 CCTGGAGGGTCCTGTACAATCTCATCATGGGACTCCTGCCCTTACCCAGGGGCCACAGAGCCCCCGAGATGGAGCCCAA TTAG Bcl2 NM_000633 CAGATGGACCTAGTACCCACTGAGATTTCCACGCCGAAGGACAGCGATGGGAAAAATGCCCTTAAATCATAGG CA9 NM_001216 ATCCTAGCCCTGGTTTTTGGCCTCCTTTTTGCTGTCACCAGCGTCGCGTTCCTTGTGCAGATGAGAAGGCAG CCNB1 NM_031966 TTCAGGTTGTTGCAGGAGACCATGTACATGACTGTCTCCATTATTGATCGGTTCATGCAGAATAATTGTGTGCCCAAGAA GATG CCND1 NM_001758 GCATGTTCGTGGCCTCTAAGATGAAGGAGACCATCCCCCTGACGGCCGAGAAGCTGTGCATCTACACCG CCNE1 NM_001238 AAAGAAGATGATGACCGGGTTTACCCAAACTCAACGTGCAAGCCTCGGATTATTGCACCATCCAGAGGCTC CCNE2 NM_057749 ATGCTGTGGCTCCTTCCTAACTGGGGCTTTCTTGACATGTAGGTTGCTTGGTAATAACCTTTTTGTATATCACAATTTGGGT CD3z NM_000734 AGATGAAGTGGAAGGCGCTTTTCACCGCGGCCATCCTGCAGGCACAGTTGCCGATTACAGAGGCA CD68 NM_001251 TGGTTCCCAGCCCTGTGTCCACCTCCAAGCCCAGATTCAGATTCGAGTCATGTACACAACCCAGGGTGGAGGAG CD9 NM_001769 GGGCGTGGAACAGTTTATCTCAGACATCTGCCCCAAGAAGGACGTACTCGAAACCTTCACCGTG CDH1 NM_004360 TGAGTGTCCCCCGGTATCTTCCCCGCCCTGCCAATCCCGATGAAATTGGAAATTTTATTGATGAAAATCTGAAAGCGGCTG CEGP1 NM_020974 TGACAATCAGCACACCTGCATTCACCGCTCGGAAGAGGGCCTGAGCTGCATGAATAAGGATCACGGCTGTAGTCACA Chk1 NM_001274 GATAAATTGGTACAAGGGATCAGCTTTTCCCAGCCCACATGTCCTGATCATATGCTTTTGAATAGTCAGTTACTTGGCACCC CIAP1 NM_001166 TGCCTGTGGTGGGAAGCTCAGTAACTGGGAACCAAAGGATGATGCTATGTCAGAACACCGGAGGCATTTTCC cIAP2 NM_001165 GGATATTTCCGTGGCTCTTATTCAAACTCTCCATCAAATCCTGTAAACTCCAGAGCAAATCAAGATTTTTCTGCCTTGATGA GAAG cMet NM_000245 GACATTTCCAGTCCTGCAGTCAATGCCTCTCTGCCCCACCCTTTGTTCAGTGTGGCTGGTGCCACGACAAATGTGTGCGATC GGAG Contig 278 AK000618 GGCATCCTGGCCCAAAGTTTCCCAAATCCAGGCGGCTAGAGGCCCACTGCTTCCCAACTACCAGCTGAGGGGGTC COX2 NM_000963 TCTGCAGAGTTGGAAGCACTCTATGGTGACATCGATGCTGTGGAGCTGTATCCTGCCCTTCTGGTAGAAAAGCCTCGGC CTSL NM_001912 GGGAGGCTTATCTCACTGAGTGAGCAGAATCTGGTAGACTGCTCTGGGCCTCAAGGCAATGMGGCTGCAATGG CTSL2 NM_001333 TGTCTCACTGAGCGAGCAGAATCTGGTGGACTGTTCGCGTCCTCAAGGCAATCAGGGCTGCAATGGT DAPK1 NM_004938 CGCTGACATCATGAATGTTCCTCGACCGGCTGGAGGCGAGTTTGGATATGACAAAGACACATCGTTGCTGAAAGAGA DIABLO NM_019887 CACAATGGCGGCTCTGAAGAGTTGGCTGTCGCGCAGCGTAACTTCATTCTTCAGGTACAGACAGTGTTTGTGT DR5 NM_003842 CTCTGAGACAGTGCTTCGATGACTTTGCAGACTTGGTGCCCTTTGACTCCTGGGAGCCGCTCATGAGGAAGTTGGGCCTCAT GG EGFR NM_005228 TGTCGATGGACTTCCAGAACCACCTGGGCAGCTGCCAAAAGTGTGATCCAAGCTGTCCCAAT EIF4E NM_001968 GATCTAAGATGGCGACTGTCGAACCGGAAACCACCCCTACTCCTAATCCCCCGACTACAGAAGAGGAGAAAACGGAATCTAA EMS1 NM_005231 GGCAGTGTCACTGAGTCCTTGAAATCCTCCCCTGCCCCGCGGGTCTCTGGATTGGGACGCACAGTGCA EpCAM NM_002354 GGGCCCTCCAGAACAATCATGGGCTTTATGATCCTGACTGCGATGAGAGCGGGCTCTTTAAGGCCAAGCAGTGCA EPHX1 NM_000120 ACCGTAGGCTCTGCTCTGAATGACTCTCCTGTGGGTCTGGCTGCCTATATTCTAGAGAAGTTTTCCACCTGGACCA ErbB3 NM_001982 CGGTTATGTCATGCCAGATACACACCTCAAAGGTACTCCCTCCTCCCGGGAAGGCACCCTTTCTTCAGTGGGTCTCAGTTC EstR1 NM_000125 CGTGGTGCCCCTCTATGACCTGCTGCTGGAGATGCTGGACGCCCACCGCCTACATGCGCCCACTAGCC FBXO5 NM_012177 GGCTATTCCTCATTTTCTCTACAAAGTGGCCTCAGTGAACATGAAGAAGGTAGCCTCCTGGAGGAGAATTTCGGTGACAGTC TACAATCC FGF18 NM_003862 CGGTAGTCAAGTCCGGATCAACGGCAAGGAGACGGAATTCTACCTGTGCATGAACCGCAAAGGCAAGC FGFR1 NM_023109 CACGGGACATTCACCACATCGACTACTATAAAAAGACAACCAACGGCCGACTGCCTGTGAAGTGGATGGCACCC FHIT NM_002012 CCAGTGGAGCGCTTCCATGACCTGCGTCCTGATGAAGTGGCCGATTTGTTTCAGACGACCCAGAGAG FRP1 NM_003012 TTGGTACCTGTGGGTTAGCATCAAGTTCTCCCCAGGGTAGAATTCAATCAGAGCTCCAGTTTGCATTTGGATGTG G-Catenin NM_002230 TCAGCAGCAAGGGCATCATGGAGGAGGATGAGGCCTGCGGGCGCCAGTACACGCTCAAGAAAACCACC CAPDH NM_002046 ATTCCACCCATGGCAAATTCCATGGCACCGTCAAGGCTGAGAACGGGAAGCTTGTCATCAATGGAAATCCCATC GATA3 NM_002051 CAAAGGAGCTCACTGTGGTGTCTGTGTTCCAACCACTGAATCTGGACCCCATCTGTGAATAAGCCATTCTGACTC GR87 NM_005310 CCATCTGCATCCATCTTGTTTGGGCTCCCCACCCTTGAGAAGTGCCTCAGATAATACCCTGGTGGCC GRO1 NM_001511 CGAAAAGATGCTGAACAGTGACAAATCCAACTGACCAGAAGGGAGGAGGAAGCTCACTGGTGGCTGTTCCTGA GSTM1 NM_000561 AAGCTATGAGGAAAAGAAGTACACGATGGGGGACGCTCCTGATTATGACAGAAGCCAGTGGCTGAATGAAAAATTCAAGCTG GGCC GUS NM_000181 CCCACTCAGTAGCCAAGTCACAATGTTTGGAAAACAGCCCGTTTACTTGAGCAAGACTGATACCACCTGCGTG HER2 NM_004448 CGGTGTGAGAAGTGCAGCAAGCCCTGTGCCCGAGTGTGCTATGGTCTGGGCATGGAGCACTTGCGAGAGG HIF1A NM_001530 TGAACATAAAGTCTGCAACATGGAAGGTATTGCACTGCACAGGCCACATTCACGTATATGATACCAACAGTAACCAACCTCA HNF3A NM_004496 TCCAGGATGTTAGGAACTGTGAAGATGGAAGGGCATGAAACCAGCGACTGGAACAGCTACTACGCAGACACGC ID1 NM_002165 AGAACCGCAAGGTGAGCAAGGTGGAGATTCTCCAGCACGTCATCGACTACATCAGGGACCTTCAGTTGGA IGF1 NM_000618 TCCGGAGCTGTGATCTAAGGAGGCTGGAGATGTATTGCGCACCCCTCAAGCCTGCCAAGTCAGCTCGCTCTGTCCG IGF1R NM_000875 GCATGGTAGCCGAAGATTTCACAGTCAAAATCGGAGATTTTGGTATGACGCGAGATATCTATGAGACAGACTATTACCG GAAA IGFBP2 NM_000597 GTGGACAGCACCATGAACATGTTGGGCGGGGGAGGCAGTGCTGGCCGGAAGCCCCTCAAGTCGGGTATGAAGG IL6 NM_000600 CCTGAACCTTCCAAAGATGGCTGAAAAAGATGGATGCTTCCAATCTGGATTCAATGAGGAGACTTGCCTGGT IRS1 NM_005544 CCACAGCTCACCTTCTGTCAGGTGTCCATCCCAGCTCCAGCCAGCTCCCAGAGAGGAAGAGACTGGCACTGAGG Ki-67 NM_002417 CGGACTTTGGGTGCGACTTGACGAGCGGTGGTTCGACAAGTGGCCTTGCGGGCCGGATCGTCCCAGTGGAAGAGTTGTAA KLK10 NM_002776 GCCCAGAGGCTCCATCGTCCATCCTCTTCCTCCCCAGTCGGCTGAACTCTCCCCTTGTCTGCACTGTTCAAACCTCTG KRT14 NM_000526 GGCCTGCTGAGATCAAAGACTACAGTCCCTACTTCAAGACCATTGAGGACCTGAGGAACAAGATTCTCACAGCCACAG TGGAC KRT17 NM_000422 CGAGGATTGGTTCTTCAGCAAGACAGAGGAACTGAACCGCGAGGTGGCCACCAACAGTGAGCTGGTGCAGAGT KRT18 NM_000224 AGAGATCGAGGCTCTCAAGGAGGAGCTGCTCTTCATGAAGAAGAACCACGAAGAGGAAGTAAAAGGCC KRT19 NM_002276 TGAGCGGCAGAATCAGGAGTACCAGCGGCTCATGGACATCAAGTCGCGGCTGGAGCAGGAGATTGCCACCTACCGCA KRT5 NM_000424 TCAGTGGAGAAGGAGTTGGACCAGTCAACATCTCTGTTGTCACAAGCAGTGTTTCCTCTGGATATGGCA KRT8 NM_002273 GGATGAAGCTTACATGAACAAGGTAGAGCTGGAGTCTCGCCTGGAAGGGCTGACCGACGAGATCAACTTCCTCAGGCAGCTA TATG LOT1 varia NM_002656 GGAAAGACCACCTGAAAAACCACCTCCAGACCCACGACCCCAACAAAATGGCCTTTGGGTGTGAGGAGTGTGGGAAGAA GTAC Maspin NM_002639 CAGATGGCCACTTTGAGAACATTTTAGCTGACAACAGTGTGAACGACCAGACCAAAATCCTTGTGGTTAATGCTGCC MCM2 NM_004526 GACTTTTGCCCCGCTACCTTTCATTTCCGGCGTGACAACAATGAGCTGTTGCTCTTCATACTGAAGCAGTTAGTGGC MCM3 NM_002388 GGAGAACAATCCCCTTGAGACAGAATATGGCCTTTCTGTCTACAAGGATCACCAGACCATCACCATCCAGGAGAT MCM6 NM_005915 TGATGGTCCTATGTGTCACATTCATCACAGGTTTCATACCAACACAGGCTTCAGCACTTCCTTTGGTGTGTTTCCTGTCCCA MDM2 NM_002392 CTACAGGGACGCCATCGAATCCGGATCTTGATGCTGGTGTAAGTGAACATTCAGGTGATTGGTTGGAT MMP9 NM_004994 GAGAACCAATCTCACCGACAGGCAGCTGGCAGAGGAATACCTGTACCGCTATGGTTACACTCGGGTG MTA1 NM_004689 CCGCCCTCACCTGAAGAGAAACGCGCTCCTTGGCGGACACTGGGGGAGGAGAGGAAGAAGCGCGGCTAACTTATTCC MYBL2 NM_002466 GCCGAGATCGCCAAGATGTTGCCAGGGAGGACAGACAATGCTGTGAAGAATCACTGGAACTCTACCATCAAAAG P14ARF S78535 CCCTCGTGCTGATGCTACTGAGGAGCCAGCGTCTAGGGCAGCAGCCGCTTCCTAGAAGACCAGGTCATGATG p27 NM_004064 CGGTGGACCACGAAGAGTTAACCCGGGACTTGGAGAAGCACTGCAGAGACATGGAAGAGGCGAGCC P53 NM_000546 CTTTGAACCCTTGCTTGCAATAGGTGTGCGTCAGAAGCACCCAGGACTTCCATTTGCTTTGTCCCGGG PAI1 NM_000602 CCGCAACGTGGTTTTCTCACCCTATGGGGTGGCCTCGGTGTTGGCCATGCTCCAGCTGACAACAGGAGGAGAAACCCAGCA PDGFRb NM_002609 CCAGCTCTCCTTCCAGCTACAGATCAATGTCCCTGTCCGAGTGCTGGAGCTAAGTGAGAGCCACCC PI3KC2A NM_002645 ATACCAATCACCGCACAAACCCAGGCTATTTGTTAAGTCCAGTCACAGCGCAAAGAAACATATGCGGAGAAAATGCTA GTGTG PPM1D NM_003620 GCCATCCGCAAAGGCTTTCTCGCTTGTCACCTTGCCATGTGGAAGAAACTGGCGGAATGGCC PR NM_000926 GCATCAGGCTGTCATTATGGTGTCCTTACCTGTGGGAGCTGTAAGGTCTTCTTTAAGAGGGCAATGGAAGGGCAGCACAACT ACT PRAME NM_006115 TCTCCATATCTGCCTTGCAGAGTCTCCTGCAGCACCTCATCGGGCTGAGCAATCTGACCCACCTGC pS2 NM_003225 GCCCTCCCAGTGTGCAAATAAGGGCTGCTGTTTCGACGACACCGTTCGTGGGGTCCCCTGGTGCTTCTATCCTAATACCATC GACG RAD51C NM_058216 GAACTTCTTGAGCAGGAGCATACCCAGGGCTTCATAATCACCTTCTGTTCAGCACTAGATGATATTCTTGGGGGTGGA RB1 NM_000321 CGAAGCCCTTACAAGTTTCCTAGTTCACCCTTACGGATTCCTGGAGGGAACATCTATATTTCACCCCTGAAGAGTCC RIZ1 NM_012231 CCAGACGAGCGATTAGAAGCGGCAGCTTGTGAGGTGAATGATTTGGGGGAAGAGGAGGAGGAGGAAGAGGAGGA STK15 NM_003600 CATCTTCCAGGAGGACCACTCTCTGTGGCACCCTGGACTACCTGCCCCCTGAAATGATTGAAGGTCGGA STMY3 NM_005940 CCTGGAGGCTGCAACATACCTCAATCCTGTCCCAGGCCGGATCCTCCTGAAGCCCTTTTCGCAGCACTGCTATCCTCCAAAG CCATTGTA

[0210] TABLE 5B SURV NM_001168 TGTTTTGATTCCCGGGCTTACCAGGTGAGAAGTGAGGGAGGAAGAAGGCAGTGTCCCTTTTGCTAGAGCTGACAGCTTTG TBP NM_003194 GCCCGAAACGCCGAATATAATCCCAAGCGGTTTGCTGCGGTAATCATGAGGATAAGAGAGCCACG TGFA NM_003236 GGTGTGCCACAGACCTTCCTACTTGGCCTGTAATCACCTGTGCAGCCTTTTGTGGGCCTTCAAAACTCTGTCAAGAACTCCGT TIMP 1 NM_003254 TCCCTGCGGTCCCAGATAGCCTGAATCCTGCCCGGAGTGGAACTGAAGCCTGCACAGTGTCCACCCTGTTTCCCAC TOP2A NM_001067 AATCCAAGGGGGAGAGTGATGACTTCCATATGGACTTTGACTCAGCTGTGGCTCCTCGGGCAAAATCTGTAC TOP2B NM_001068 TGTGGACATCTTCCCCTCAGACTTCCCTACTGAGCCACCTTCTCTGCCACGAACCGGTCGGGCTAG TP NM_001953 CTATATGCAGCCAGAGATGTGACAGCCACCGTGGACAGCCTGCCACTCATCACAGCCTCCATTCTCAGTAAGAAACTCGTGG TP538P2 NM_005426 GGGCCAAATATTCAGAAGCTTTTATATCAGAGGACCACCATAGCGGCCATGGAGACCATCTCTGTCCCATCATACCCATCC TRAIL NM_003810 CTTCACAGTGCTCCTGCAGTCTCTCTGTGTGGCTGTAACTTACGTGTACTTTACCAACGAGCTGAAGCAGATG TS NM_001071 GCCTCGGTGTGCCTTTCAACATCGCCAGCTACGCCCTGCTCACGTACATGATTGCGCACATCACG upa NM_002658 GTGGATGTGCCCTGAAGGACAAGCCAGGCGTCTACACGAGAGTCTCACACTTCTTACCCTGGATCCGCAG VDR NM_000376 GCCCTGGATTTCAGAAAGAGCCAAGTCTGGATCTGGGACCCTTTCCTTCCTTCCCTGGCTTGTAACT VEGF NM_003376 CTGCTGTCTTGGGTGCATTGGAGCCTTGCCTTGCTGCTCTACCTCCACCATGCCAAGTGGTCCCAGGCTGC VEGPB NM_003377 TGACGATGGCCTGGAGTGTGTGCCCACTGGGCAGCACCAAGTCCGGATGCAGATCCTCATGATCCGGTACC WISP1 NM_003882 AGAGGCATCCATGAACTTTCACACTTGCGGGCTGCATCAGCACACGCTCCTATCAACCCAAGTACTGTGGAGTTTG XIAP NM_001167 GCAGTTGGAAGACACAGGAAAGTATCCCCAAATTGCAGATTTATCAACGGCTTTTATCTTGAAAATAGTGCCACGCA YB-1 NM_004559 AGACTGTGGAGTTTGATGTTGTTGAAGGAGAAAAGGGTGCGGAGGCAGCAAATGTTACAGGTCCTGGTGGTGTTCC ZNF217 NM_006526 ACCCAGTAGCAAGGAGAAGCCCACTCACTGCTCCGAGTGCGGCAAAGCTTTCAGAACCTACCACCAGCTG

[0211] TABLE 6A Gene Accession Probe Name Seq Len AIB1 NM_006534 S1994/AIB1.f3 GCGGCGAGTTTCCGATTTA 19 AIB1 NM_006534 S1995/AIB1.r3 TGAGTCCACCATCCAGCAAGT 21 AIB1 NM_006534 S5055/AIB1.p3 ATGGCGGCGGGAGGATCAAAA 21 AKT1 NM_005163 S0010/AKT1.f3 CGCTTCTATGGCGCTGAGAT 20 AKT1 NM_005163 S0012/AKT1.r3 TCCCGGTACACCACGTTCTT 20 AKT1 NM_005163 S4776/AKT1.p3 CAGCCCTGGACTACCTGCACTCGG 24 AKT2 NM_001626 S0828/AKT2.f3 TCCTGCCACCCTTCAAACC 19 AKT2 NM_001626 S0829/AKT2.r3 GGCGGTAAATTCATCATCGAA 21 AKT2 NM_001626 S4727/AKT2.p3 CAGGTCACGTCCGAGGTCGACACA 24 APC NM_000038 S0022/APC.f4 GGACAGCAGGAATGTGTTTC 20 APC NM_000038 S0024/APC.r4 ACCCACTCGATTTGTTTCTG 20 APC NM_000038 S4888/APC.p4 CATTGGCTCCCCGTGACCTGTA 22 AREG NM_001657 S0025/AREG.f2 TGTGAGTGAAATGCCTTCTAGTAGTGA 27 AREG NM_001657 S0027/AREG.r2 TTGTGGTTCGTTATCATACTCTTCTGA 27 AREG NM_001657 S4889/AREG.p2 CCGTCCTCGGGAGCCGACTATGA 23 B-actin NM_001101 S0034/B-acti.f2 CAGCAGATGTGGATCAGCAAG 21 B-actin NM_001101 S0036/B-acti.r2 GCATTTGCGGTGGACGAT 18 B-actin NM_001101 S4730/B-acti.p2 AGGAGTATGACGAGTCCGGCCCC 23 B-Catenin NM_001904 S2150/B-Cate.f3 GGCTCTTGTGCGTACTGTCCTT 22 B-Catenin NM_001904 S2151/B-Cate.r3 TCAGATGACGAAGAGCACAGATG 23 B-Catenin NM_001904 S5046/B-Cate.p3 AGGCTCAGTGATGTCTTCCCTGTCACCAG 29 BAD NM_032989 S2011/BAD.f1 GGGTCAGGTGCCTCGAGAT 19 BAD NM_032989 S2012/BAD.r1 CTGCTCACTCGGCTCAAACTC 21 BAD NM_032989 S5058/BAD.p1 TGGGCCCAGAGCATGTTCCAGATC 24 BAG1 NM_004323 S1386/BAG1.f2 CGTTGTCAGCACTTGGAATACAA 23 BAG1 NM_004323 S1387/BAG1.r2 GTTCAACCTCTTCCTGTGGACTGT 24 BAG1 NM_004323 S4731/BAG1.p2 CCCAATTAACATGACCCGGCAACCAT 26 BBC3 NM_014417 S1584/BBC3.f2 CCTGGAGGGTCCTGTACAAT 20 BBC3 NM_014417 S1585/BBC3.r2 CTAATTGGGCTCCATCTCG 19 BBC3 NM_014417 S4890/BBC3.p2 CATCATGGGACTCCTGCCCTTACC 24 Bcl2 NM_000633 S0043/Bcl2.f2 CAGATGGACCTAGTACCCACTGAGA 25 Bcl2 NM_000633 S0045/Bcl2.r2 CCTATGATTTAAGGGCATTTTTCC 24 Bcl2 NM_000633 S4732/Bcl2.p2 TTCCACGCCGAAGGACAGCGAT 22 CA9 NM_001216 S1398/CA9.f3 ATCCTAGCCCTGGTTTTTGG 20 CA9 NM_001216 S1399/CA9.r3 CTGCCTTCTCATCTGCACAA 20 CA9 NM_001216 S4938/CA9.p3 TTTGCTGTCACCAGCGTCGC 20 CCNB1 NM_031966 S1720/CCNB1.f2 TTCAGGTTGTTGCAGGAGAC 20 CCNB1 NM_031966 S1721/CCNB1.r2 CATCTTCTTGGGCACACAAT 20 CCNB1 NM_031966 S4733/CCNB1.p2 TGTCTCCATTATTGATCGGTTCATGCA 27 CCND1 NM_001758 S0058/CCND1.f3 GCATGTTCGTGGCCTCTAAGA 21 CCND1 NM_001758 S0060/CCND1.r3 CGGTGTAGATGCACAGCTTCTC 22 CCND1 NM_001758 S4986/CCND1.p3 AAGGAGACCATCCCCCTGACGGC 23 CCNE1 NM_001238 S1446/CCNE1.f1 AAAGAAGATGATGACCGGGTTTAC 24 CCNE1 NM_001238 S1447/CCNE1.r1 GAGCCTCTGGATGGTGCAAT 20 CCNE1 NM_001238 S4944/CCNE1.p1 CAAACTCAACGTGCAAGCCTCGGA 24 CCNE2 NM_057749 S1458/CCNE2.f2 ATGCTGTGGCTCCTTCCTAACT 22 CCNE2 NM_057749 S1459/CCNE2.r2 ACCCAAATTGTGATATACAAAAAGGTT 27 CCNE2 NM_057749 S4945/CCNE2.p2 TACCAAGCAACCTACATGTCAAGAAAGCCC 30 CD3z NM_000734 S0064/CD3z.f1 AGATGAAGTGGAAGGCGCTT 20 CD3z NM_000734 S0066/CD3z.r1 TGCCTCTGTAATCGGCAACTG 21 CD3z NM_000734 S4988/CD3z.p1 CACCGCGGCCATCCTGCA 18 CD68 NM_001251 S0067/CD68.f2 TGGTTCCCAGCCCTGTGT 18 CD68 NM_001251 S0069/CD68.r2 CTCCTCCACCCTGGGTTGT 19 CD68 NM_001251 S4734/CD68.p2 CTCCAAGCCCAGATTCAGATTCGAGTCA 28 CD9 NM_001769 S0686/CD9.f1 GGGCGTGGAACAGTTTATCT 20 CD9 NM_001769 S0687/CD9.r1 CACGGTGAAGGTTTCGAGT 19 CD9 NM_001769 S4792/CD9.p1 AGACATCTGCCCCAAGAAGGACGT 24 CDH1 NM_004360 S0073/CDH1.f3 TGAGTGTCCCCCGGTATCTTC 21 CDH1 NM_004360 S0075/CDH1.r3 CAGCCGCTTTCAGATTTTCAT 21 CDH1 NM_004360 S4990/CDH1.p3 TGCCAATCCCGATGAAATTGGAAATTT 27 CEGP1 NM_020974 S1494/CEGP1.f2 TGACAATCAGCACACCTGCAT 21

[0212] TABLE 6B CEGP1 NM_020974 S1495/CEGP1.r2 TGTGACTACAGCCGTGATCCTTA 23 CEGP1 NM_020974 S4735/CEGP1.p2 CAGGCCCTCTTCCGAGCGGT 20 Chk1 NM_001274 S1422/Chk1.f2 GATAAATTGGTACAAGGGATCAGCTT 26 Chk1 NM_001274 S1423/Chk1.r2 GGGTGCCAAGTAACTGACTATTCA 24 Chk1 NM_001274 S4941/Chk1.p2 CCAGCCCACATGTCCTGATCATATGC 26 CIAP1 NM_001166 S0764/CIAP1.f2 TGCCTGTGGTGGGAAGCT 18 CIAP1 NM_001166 S0765/CIAP1.r2 GGAAAATGCCTCCGGTGTT 19 CIAP1 NM_001166 S4802/CIAP1.p2 TGACATAGCATCATCCTTTGGTTCCCAGTT 30 cIAP2 NM_001165 S0076/cIAP2.f2 GGATATTTCCGTGGCTCTTATTCA 24 cIAP2 NM_001165 S0078/cIAP2.r2 CTTCTCATCAAGGCAGAAAAATCTT 25 cIAP2 NM_001165 S4991/cIAP2.p2 TCTCCATCAAATCCTGTAAACTCCAGAGCA 30 cMet NM_000245 S0082/cMet.f2 GACATTTCCAGTCCTGCAGTCA 22 cMet NM_000245 S0084/cMet.r2 CTCCGATCGCACACATTTGT 20 cMet NM_000245 S4993/cMet.p2 TGCCTCTCTGCCCCACCCTTTGT 23 Contig 27882 AK000618 S2633/Contig.f3 GGCATCCTGGCCCAAAGT 18 Contig 27882 AK000618 S2634/Contig.r3 GACCCCCTCAGCTGGTAGTTG 21 Contig 27882 AK000618 S4977/Contig.p3 CCCAAATCCAGGCGGCTAGAGGC 23 COX2 NM_000963 S0088/C0X2.f1 TCTGCAGAGTTGGAAGCACTCTA 23 COX2 NM_000963 S0090/COX2.r1 GCCGAGGCTTTTCTACCAGAA 21 COX2 NM_000963 S4995/COX2.p1 CAGGATACAGCTCCACAGCATCGATGTC 28 CTSL NM_001912 S1303/CTSL.f2 GGGAGGCTTATCTCACTGAGTGA 23 CTSL NM_001912 S1304/CTSL.r2 CCATTGCAGCCTTCATTGC 19 CTSL NM_001912 S4899/CTSL.p2 TTGAGGCCCAGAGCAGTCTACCAGATTCT 29 CTSL2 NM_001333 S4354/CTSL2.f1 TGTCTCACTGAGCGAGCAGAA 21 CTSL2 NM_001333 S4355/CTSL2.r1 ACCATTGCAGCCCTGATTG 19 CTSL2 NM_001333 S4356/CTSL2.p1 CTTGAGGACGCGAACAGTCCACCA 24 DAPK1 NM_004938 S1768/DAPK1.f3 CGCTGACATCATGAATGTTCCT 22 DAPK1 NM_004938 S1769/DAPK1.r3 TCTCTTTCAGCAACGATGTGTCTT 24 DAPK1 NM_004938 S4927/DAPK1.p3 TCATATCCAAACTCGCCTCCAGCCG 25 DIABLO NM_019887 S0808/DIABLO.f1 CACAATGGCGGCTCTGAAG 19 DIABLO NM_019887 S0809/DIABLO.r1 ACACAAACACTGTCTGTACCTGAAGA 26 DIABLO NM_019887 S4813/DIABLO.p1 AAGTTACGCTGCGCGACAGCCAA 23 DR5 NM_003842 S2551/DR5.f2 CTCTGAGACAGTGCTTCGATGACT 24 DR5 NM_003842 S2552/DR5.r2 CCATGAGGCCCAACTTCCT 19 DR5 NM_003842 S4979/DR5.p2 CAGACTTGGTGCCCTTTGACTCC 23 EGFR NM_005228 S0103/EGFR.f2 TGTCGATGGACTTCCAGAAC 20 EGFR NM_005228 S0105/EGFR.r2 ATTGGGACAGCTTGGATCA 19 EGFR NM_005228 S4999/EGFR.p2 CACCTGGGCAGCTGCCAA 18 EIF4E NM_001968 S0106/EIF4E.f1 GATCTAAGATGGCGACTGTCGAA 23 EIF4E NM_001968 S0108/EIF4E.r1 TTAGATTCCGTTTTCTCCTCTTCTG 25 EIF4E NM_001968 S5000/EIF4E.p1 ACCACCCCTACTCCTAATCCCCCGACT 27 EMS1 NM_005231 S2663/EMS1.f1 GGCAGTGTCACTGAGTCCTTGA 22 EMS1 NM_005231 S2664/EMS1.r1 TGCACTGTGCGTCCCAAT 18 EMS1 NM_005231 S4956/EMS1.p1 ATCCTCCCCTGCCCCGCG 18 EpCAM NM_002354 S1807/EpCAM.f1 GGGCCCTCCAGAACAATGAT 20 EpCAM NM_002354 S1808/EpCAM.r1 TGCACTGCTTGGCCTTAAAGA 21 EpCAM NM_002354 S4984/EpCAM.p1 CCGCTCTCATCGCAGTCAGGATCAT 25 EPHX1 NM_000120 S1865/EPHX1.f2 ACCGTAGGCTCTGCTCTGAA 20 EPHX1 NM_000120 S1866/EPHX1.r2 TGGTCCAGGTGGAAAACTTC 20 EPHX1 NM_000120 S4754/EPHX1.p2 AGGCAGCCAGACCCACAGGA 20 ErbB3 NM_001982 S0112/ErbB3.f1 CGGTTATGTCATGCCAGATACAC 23 ErbB3 NM_001982 S0114/ErbB3.r1 GAACTGAGACCCACTGAAGAAAGG 24 ErbB3 NM_001982 S5002/ErbB3.p1 CCTCAAAGGTACTCCCTCCTCCCGG 25 EstR1 NM_000125 S0115/EstR1.f1 CGTGGTGCCCCTCTATGAC 19 EstR1 NM_000125 S0117/EstR1.r1 GGCTAGTGGGCGCATGTAG 19 EstR1 NM_000125 S4737/EstR1.p1 CTGGAGATGCTGGACGCCC 19 FBXO5 NM_012177 S2017/FBXO5.r1 GGATTGTAGACTGTCACCGAAATTC 25 FBXO5 NM_012177 S2018/FBXO5.f1 GGCTATTCCTCATTTTCTCTACAAAGTG 28 FBXO5 NM_012177 S5061/FBXO5.p1 CCTCCAGGAGGCTACCTTCTTCATGTTCAC 30 FGF18 NM_003862 S1665/FGF18.f2 CGGTAGTCAAGTCCGGATCAA 21 FGF18 NM_003862 S1666/FGF18.r2 GCTTGCCTTTGCGGTTCA 18 FGF18 NM_003862 S4914/FGF18.p2 CAAGGAGACGGAATTCTACCTGTGC 25

[0213] TABLE 6C FGFR1 NM_023109 S0818/FGFR1.f3 CACGGGACATTCACCACATC 20 FGFR1 NM_023109 S0819/FGFR1.r3 GGGTGCCATCCACTTCACA 19 FGFR1 NM_023109 S4816/FGFR1.p3 ATAAAAAGACAACCAACGGCCGACTGC 27 FHIT NM_002012 S2443/FHIT.f1 CCAGTGGAGCGCTTCCAT 18 FHIT NM_002012 S2444/FHIT.r1 CTCTCTGGGTCGTCTGAAACAA 22 FHIT NM_002012 S2445/FHIT.p1 TCGGCCACTTCATCAGGACGCAG 23 FHIT NM_002012 S4921/FHIT.p1 TCGGCCACTTCATCAGGACGCAG 23 FRP1 NM_003012 S1804/FRP1.f3 TTGGTACCTGTGGGTTAGCA 20 FRP1 NM_003012 S1805/FRP1.r3 CACATCCAAATGCAAACTGG 20 FRP1 NM_003012 S4983/FRP1.p3 TCCCCAGGGTAGAATTCAATCAGAGC 26 G-Catenin NM_002230 S2153/G-Cate.f1 TCAGCAGCAAGGGCATCAT 19 G-Catenin NM_002230 S2154/G-Cate.r1 GGTGGTTTTCTTGAGCGTGTACT 23 G-Catenin NM_002230 S5044/G-Cate.p1 CGCCCGCAGGCCTCATCCT 19 GAPDH NM_002046 S0374/GAPDH.f1 ATTCCACCCATGGCAAATTC 20 GAPDH NM 002046 S0375/GAPDH.r1 GATGGGATTTCCATTGATGACA 22 GAPDH NM_002046 S4738/GAPDH.p1 CCGTTCTCAGCCTTGACGGTGC 22 GATA3 NM_002051 S0127/GATA3.f3 CAAAGGAGCTCACTGTGGTGTCT 23 GATA3 NM_002051 S0129/GATA3.r3 GAGTCAGAATGGCTTATTCACAGATG 26 GATA3 NM_002051 SS005/GATA3.p3 TGTTCCAACCACTGAATCTGGACC 24 GRB7 NM_005310 S0130/GRB7.f2 CCATCTGCATCCATCTTGTT 20 GRB7 NM_005310 S0132/GRB7.r2 GGCCACCAGGGTATTATCTG 20 GRB7 NM_005310 S4726/GRB7.p2 CTCCCCACCCTTGAGAAGTGCCT 23 GRO1 NM_001511 S0133/GRO1.f2 CGAAAAGATGCTGAACAGTGACA 23 GRO1 NM_001511 S0135/GRO1.r2 TCAGGAACAGCCACCAGTGA 20 GRO1 NM_001511 S5006/GRO1.p2 CTTCCTCCTCCCTTCTGGTCAGTTGGAT 28 GSTM1 NM_000561 S2026/GSTM1.r1 GGCCCAGCTTGAATTTTTCA 20 GSTM1 NM_000561 S2027/GSTM1.f1 AAGCTATGAGGAAAAGAAGTACACGAT 27 GSTM1 NM_000561 S4739/GSTM1.p1 TCAGCCACTGGCTTCTGTCATAATCAGGAG 30 GUS NM_000181 S0139/GUS.f1 CCCACTCAGTAGCCAAGTCA 20 GUS NM_000181 S0141/GUS.r1 CACGCAGGTGGTATCAGTCT 20 GUS NM_000181 S4740/GUS.p1 TCAAGTAAACGGGCTGTTTTCCAAACA 27 HER2 NM_004448 S0142/HER2.f3 CGGTGTGAGAAGTGCAGCAA 20 HER2 NM_004448 S0144/HER2.r3 CCTCTCGCAAGTGCTCCAT 19 HER2 NM_004448 S4729/HER2.p3 CCAGACCATAGCACACTCGGGCAC 24 HIF1A NM_001530 S1207/HIF1A.f3 TGAACATAAAGTCTGCAACATGGA 24 HIF1A NM_001530 S1208/HIF1A.r3 TGAGGTTGGTTACTGTTGGTATCATATA 28 HIF1A NM_001530 S4753/HIF1A.p3 TTGCACTGCACAGGCCACATTCAC 24 HNF3A NM_004496 S0148/HNF3A.f1 TCCAGGATGTTAGGAACTGTGAAG 24 HNF3A NM_004496 S0150/HNF3A.r1 GCGTGTCTGCGTAGTAGCTGTT 22 HNF3A NM_004496 S5008/HNF3A.p1 AGTCGCTGGTTTCATGCCCTTCCA 24 ID1 NM_002165 S0820/ID1.f1 AGAACCGCAAGGTGAGCAA 19 ID1 NM_002165 S0821/ID1.r1 TCCAACTGAAGGTCCCTGATG 21 ID1 NM_002165 S4832/ID1.p1 TGGAGATTCTCCAGCACGTCATCGAC 26 IGF1 NM_000618 S0154/IGF1.f2 TCCGGAGCTGTGATCTAAGGA 21 IGF1 NM_000618 S0156/IGF1.r2 CGGACAGAGCGAGCTGACTT 20 IGF1 NM_000618 S5010/IGF1.p2 TGTATTGCGCACCCCTCAAGCCTG 24 IGF1R NM_000875 S1249/IGF1R.f3 GCATGGTAGCCGAAGATTTCA 21 IGF1R NM_000875 S1250/IGF1R.r3 TTTCCGGTAATAGTCTGTCTCATAGATATC 30 IGF1R NM_000875 S4895/IGF1R.p3 CGCGTCATACCAAAATCTCCGATTTTGA 28 IGFBP2 NM_000597 S1128/IGFBP2.f1 GTGGACAGCACCATGAACA 19 IGFBP2 NM_000597 S1129/IGFBP2.r1 CCTTCATACCCGACTTGAGG 20 IGFBP2 NM_000597 S4837/IGFBP2.p1 CTTCCGGCCAGCACTGCCTC 20 IL6 NM_000600 S0760/IL6.f3 CCTGAACCTTCCAAAGATGG 20 IL6 NM_000600 S0761/IL6.r3 ACCAGGCAAGTCTCCTCATT 20 IL6 NM_000600 S4800/IL6.p3 CCAGATTGGAAGCATCCATCTTTTTCA 27 IRS1 NM_005544 S1943/IRS1.f3 CCACAGCTCACCTTCTGTCA 20 IRS1 NM_005544 S1944/IRS1.r3 CCTCAGTGCCAGTCTCTTCC 20 IRS1 NM_005544 S5050/IRS1.p3 TCCATCCCAGCTCCAGCCAG 20 Ki-67 NM_002417 S0436/Ki-67.f2 CGGACTTTGGGTGCGACTT 19 Ki-67 NM_002417 S0437/Ki-67.r2 TTACAACTCTTCCACTGGGACGAT 24 Ki-67 NM_002417 S4741/Ki-67.p2 CCACTTGTCGAACCACCGCTCGT 23 KLK10 NM_002776 S2624/KLK10.f3 GCCCAGAGGCTCCATCGT 18

[0214] TABLE 6D KLK10 NM_002776 S2625/KLK10.r3 CAGAGGTTTGAACAGTGCAGACA 23 KLK10 NM_002776 S4978/KLK10.p3 CCTCTTCCTCCCCAGTCGGCTGA 23 KRT14 NM_000526 S1853/KRT14.f1 GGCCTGCTGAGATCAAAGAC 20 KRT14 NM_000526 S1854/KRT14.r1 GTCCACTGTGGCTGTGAGAA 20 KRT14 NM_000526 S5037/KRT14.p1 TGTTCCTCAGGTCCTCAATGGTCTTG 26 KRT17 NM_000422 S0172/KRT17.f2 CGAGGATTGGTTCTTCAGCAA 21 KRT17 NM_000422 S0174/KRT17.r2 ACTCTGCACCAGCTCACTGTTG 22 KRT17 NM_000422 S5013/KRT17.p2 CACCTCGCGGTTCAGTTCCTCTGT 24 KRT18 NM_000224 S1710/KRT18.f2 AGAGATCGAGGCTCTCAAGG 20 KRT18 NM_000224 S1711/KRT18.r2 GGCCTTTTACTTCCTCTTCG 20 KRT18 NM_000224 S4762/KRT18.p2 TGGTTCTTCTTCATGAAGAGCAGCTCC 27 KRT19 NM_002276 S1515/KRT19.f3 TGAGCGGCAGAATCAGGAGTA 21 KRT19 NM_002276 S1516/KRT19.r3 TGCGGTAGGTGGCAATCTC 19 KRT19 NM_002276 S4866/KRT19.p3 CTCATGGACATCAAGTCGCGGCTG 24 KRT5 NM_000424 S0175/KRT5.f3 TCAGTGGAGAAGGAGTTGGA 20 KRT5 NM_000424 S0177/KRT5.r3 TGCCATATCCAGAGGAAACA 20 KRT5 NM_000424 S5015/KRT5.p3 CCAGTCAACATCTCTGTTGTCACAAGCA 28 KRT8 NM_002273 S2588/KRT8.f3 GGATGAAGCTTACATGAACAAGGTAGA 27 KRT8 NM_002273 S2589/KRT8.r3 CATATAGCTGCCTGAGGAAGTTGAT 25 KRT8 NM_002273 S4952/KRT8.p3 CGTCGGTCAGCCCTTCCAGGC 21 LOT1 variant 1 NM_002656 S0692/L0T1 v.f2 GGAAAGACCACCTGAAAAACCA 22 LOT1 variant 1 NM_002656 S0693/LOT1 v.r2 GTACTTCTTCCCACACTCCTCACA 24 LOT1 variant 1 NM_002656 S4793/LOT1 v.p2 ACCCACGACCCCAACAAAATGGC 23 Maspin NM_002639 S0836/Maspin.f2 CAGATGGCCACTTTGAGAACATT 23 Maspin NM_002639 S0837/Maspin.r2 GGCAGCATTAACCACAAGGATT 22 Maspin NM_002639 S4835/Maspin.p2 AGCTGACAACAGTGTGAACGACCAGACC 28 MCM2 NM_004526 S1602/MCM2.f2 GACTTTTGCCCGCTACCTTTC 21 MCM2 NM_004526 S1603/MCM2.r2 GCCACTAACTGCTTCAGTATGAAGAG 26 MCM2 NM_004526 S4900/MCM2.p2 ACAGCTCATTGTTGTCACGCCGGA 24 MCM3 NM_002388 S1524/MCM3.f3 GGAGAACAATCCCCTTGAGA 20 MCM3 NM_002388 S1525/MCM3.r3 ATCTCCTGGATGGTGATGGT 20 MCM3 NM_002388 S4870/MCM3.p3 TGGCCTTTCTGTCTACAAGGATCACCA 27 MCM6 NM_005915 S1704/MCM6.f3 TGATGGTCCTATGTGTCACATTCA 24 MCM6 NM_005915 S1705/MCM6.r3 TGGGACAGGAAACACACCAA 20 MCM6 NM_005915 S4919/MCM6.p3 CAGGTTTCATACCAACACAGGCTTCAGCAC 30 MDM2 NM_002392 S0830/MDM2.f1 CTACAGGGACGCCATCGAA 19 MDM2 NM_002392 S0831/MDM2.r1 ATCCAACCAATCACCTGAATGTT 23 MDM2 NM_002392 S4834/MDM2.p1 CTTACACCAGCATCAAGATCCGG 23 MMP9 NM_004994 S0656/MMP9.f1 GAGAACCAATCTCACCGACA 20 MMP9 NM_004994 S0657/MMP9.r1 CACCCGAGTGTAACCATAGC 20 MMP9 NM_004994 S4760/MMP9.p1 ACAGGTATTCCTCTGCCAGCTGCC 24 MTA1 NM_004689 S2369/MTA1.F1 CCGCCCTCACCTGAAGAGA 19 MTA1 NM_004689 S2370/MTA1.r1 GGAATAAGTTAGCCGCGCTTCT 22 MTA1 NM_004689 S4855/MTA1.p1 CCCAGTGTCCGCCAAGGAGCG 21 MYBL2 NM_002466 S3270/MYBL2.f1 GCCGAGATCGCCAAGATG 18 MYBL2 NM_002466 S3271/MYBL2.r1 CTTTTGATGGTAGAGTTCCAGTGATTC 27 MYBL2 NM_002466 S4742/MYBL2.p1 CAGCATTGTCTGTCCTCCCTGGCA 24 P14ARF S78535 S2842/P14ARF.f1 CCCTCGTGCTGATGCTACT 19 P14ARF S78535 S2843/P14ARF.r1 CATCATGACCTGGTCTTCTAGG 22 P14ARF S78535 S4971/P14ARF.p1 CTGCCCTAGACGCTGGCTCCTC 22 p27 NM_004064 S0205/p27.f3 CGGTGGACCACGAAGAGTTAA 21 p27 NM_004064 S0207/p27.r3 GGCTCGCCTCTTCCATGTC 19 p27 NM_004064 S4750/p27.p3 CCGGGACTTGGAGAAGCACTGCA 23 P53 NM_000546 S0208/P53.f2 CTTTGAACCCTTGCTTGCAA 20 P53 NM_000546 S0210/P53.r2 CCCGGGACAAAGCAAATG 18 P53 NM_000546 S5065/P53.p2 AAGTCCTGGGTGCTTCTGACGCACA 25 PAI1 NM_000602 S0211/PAI1.f3 CCGCAACGTGGTTTTCTCA 19 PAI1 NM_000602 S0213/PAI1.r3 TGCTGGGTTTCTCCTCCTGTT 21 PAI1 NM_000602 S5066/PAI1.p3 CTCGGTGTTGGCCATGCTCCAG 22 PDGFRb NM_002609 S1346/PDGFRb.f3 CCAGCTCTCCTTCCAGCTAC 20 PDGFRb NM_002609 S1347/PDGFRb.r3 GGGTGGCTCTCACTTAGCTC 20 PDGFRb NM_002609 S4931/PDGFRb.p3 ATCAATGTCCCTGTCCGAGTGCTG 24

[0215] TABLE 6E PI3KC2A NM_002645 S2020/PI3KC2.r1 CACACTAGCATTTTCTCCGCATA 23 PI3KC2A NM_002645 S2021/PI3KC2.f1 ATACCAATCACCGCACAAACC 21 PI3KC2A NM_002645 S5062/P13KC2.p1 TGCGCTGTGACTGGACTTAACAAATAGCCT 30 PPM1D NM_003620 S3159/PPM1D.f1 GCCATCCGCAAAGGCTTT 18 PPM1D NM_003620 S3160/PPM1D.r1 GGCCATTCCGCCAGTTTC 18 PPM1D NM_003620 S4856/PPM1D.p1 TCGCTTGTCACCTTGCCATGTGG 23 PR NM_000926 S1336/PR.f6 GCATCAGGCTGTCATTATGG 20 PR NM_000926 S1337/PR.r6 AGTAGTTGTGCTGCCCTTCC 20 PR NM_000926 S4743/PR.p6 TGTCCTTACCTGTGGGAGCTGTAAGGTC 28 PRAME NM_006115 S1985/PRAME.f3 TCTCCATATCTGCCTTGCAGAGT 23 PRAME NM_006115 S1986/PRAME.r3 GCACGTGGGTCAGATTGCT 19 PRAME NM_006115 S4756/PRAME.p3 TCCTGCAGCACCTCATCGGGCT 22 pS2 NM_003225 S0241/pS2.f2 GCCCTGCCAGTGTGCAAAT 19 pS2 NM_003225 S0243/pS2.r2 CGTCGATGGTATTAGGATAGAAGCA 25 pS2 NM_003225 S5026/pS2.p2 TGCTGTTTCGACGACACCGTTCG 23 RAD51C NM_058216 S2606/RAD51C.f3 GAACTTCTTGAGCAGGAGCATACC 24 RAD51C NM_058216 S2607/RAD51C.r3 TCCACCCCCAAGAATATCATCTAGT 25 RAD51C NM_058216 S4764/RAD51C.p3 AGGGCTTCATAATCACCTTCTGTTC 25 RB1 NM_000321 S2700/RB1.f1 CGAAGCCCTTACAAGTTTCC 20 RB1 NM_000321 S2701/RB1.r1 GGACTCTTCAGGGGTGAAAT 20 RB1 NM_000321 S4765/RB1.p1 CCCTTACGGATTCCTGGAGGGAAC 24 RIZ1 NM_012231 S1320/RIZ1.f2 CCAGACGAGCGATTAGAAGC 20 RIZ1 NM_012231 S1321/RIZ1.r2 TCCTCCTCTTCCTCCTCCTC 20 RIZ1 NM_012231 S4761/RIZ1.p2 TGTGAGGTGAATGATTTGGGGGA 23 STK15 NM_003600 S0794/STK15.f2 CATCTTCCAGGAGGACCACT 20 STK15 NM_003600 S0795/STK15.r2 TCCGACCTTCAATCATTTCA 20 STK15 NM_003600 S4745/STK15.p2 CTCTGTGGCACCCTGGACTACCTG 24 STMY3 NM_005940 S2067/STMY3.f3 CCTGGAGGCTGCAACATACC 20 STMY3 NM_005940 S2068/STMY3.r3 TACAATGGCTTTGGAGGATAGCA 23 STMY3 NM_005940 S4746/STMY3.p3 ATCCTCCTGAAGCCCTTTTCGCAGC 25 SURV NM_001168 S0259/SURV.f2 TGTTTTGATTCCCGGGCTTA 20 SURV NM_001168 S0261/SURV.r2 CAAAGCTGTCAGCTCTAGCAAAAG 24 SURV NM_001168 S4747/SURV.p2 TGCCTTCTTCCTCCCTCACTTCTCACCT 28 TBP NM_003194 S0262/TBP.f1 GCCCGAAACGCCGAATATA 19 TBP NM_003194 S0264/TBP.r1 CGTGGCTCTCTTATCCTCATGAT 23 TBP NM_003194 S4751/TBP.p1 TACCGCAGCAAACCGCTTGGG 21 TGFA NM_003236 S0489/TGFA.f2 GGTGTGCCACAGACCTTCCT 20 TGFA NM_003236 S0490/TGFA.r2 ACGGAGTTCTTGACAGAGTTTTGA 24 TGFA NM_003236 S4768/TGFA.p2 TTGGCCTGTAATCACCTGTGCAGCCTT 27 TIMP1 NM_003254 S1695/TIMP1.f3 TCCCTGCGGTCCCAGATAG 19 TIMP1 NM_003254 S1696/TIMP1.r3 GTGGGAACAGGGTGGACACT 20 TIMP1 NM_003254 S4918/TIMP1.p3 ATCCTGCCCGGAGTGGAACTGAAGC 25 TOP2A NM_001067 S0271/TOP2A.f4 AATCCAAGGGGGAGAGTGAT 20 TOP2A NM_001067 S0273/TOP2A.r4 GTACAGATTTTGCCCGAGGA 20 TOP2A NM_001067 S4777/TOP2A.p4 CATATGGACTTTGACTCAGCTGTGGC 26 TOP2B NM_001068 S0274/TOP2B.f2 TGTGGACATCTTCCCCTCAGA 21 TOP2B NM_001068 S0276/TOP2B.r2 CTAGCCCGACCGGTTCGT 18 TOP2B NM_001068 S4778/TOP2B.p2 TTCCCTACTGAGCCACCTTCTCTG 24 TP NM_001953 S0277/TP.f3 CTATATGCAGCCAGAGATGTGACA 24 TP NM_001953 S0279/TP.r3 CCACGAGTTTCTTACTGAGAATGG 24 TP NM_001953 S4779/TP.p3 ACAGCCTGCCACTCATCACAGCC 23 TP53BP2 NM_005426 S1931/TP53BP.f2 GGGCCAAATATTCAGAAGC 19 TP53BP2 NM_005426 S1932/TP53BP.r2 GGATGGGTATGATGGGACAG 20 TP53BP2 NM_005426 S5049/TP53BP.p2 CCACCATAGCGGCCATGGAG 20 TRAIL NM_003810 S2539/TRAIL.f1 CTTCACAGTGCTCCTGCAGTCT 22 TRAIL NM_003810 S2540/TRAIL.r1 CATCTGCTTCAGCTCGTTGGT 21 TRAIL NM_003810 S4980/TRAIL.p1 AAGTACACGTAAGTTACAGCCACACA 26 TS NM_001071 S0280/TS.f1 GCCTCGGTGTGCCTTTCA 18 TS NM_001071 S0282/TS.r1 CGTGATGTGCGCAATCATG 19 TS NM_001071 S4780/TS.p1 CATCGCCAGCTACGCCCTGCTC 22 upa NM_002658 S0283/upa.f3 GTGGATGTGCCCTGAAGGA 19 upa NM_002658 S0285/upa.r3 CTGCGGATCCAGGGTAAGAA 20

[0216] TABLE 6F upa NM_002658 S4769/upa.p3 AAGCCAGGCGTCTACACGAGAGTCTCAC 28 VDR NM_000376 S2745/VDR.f2 GCCCTGGATTTCAGAAAGAG 20 VDR NM_000376 S2746/VDR.r2 AGTTACAAGCCAGGGAAGGA 20 VDR NM_000376 S4962/VDR.p2 CAAGTCTGGATCTGGGACCCTTTCC 25 VEGF NM_003376 S0286/VEGF.f1 CTGCTGTCTTGGGTGCATTG 20 VEGF NM_003376 S0288/VEGF.r1 GCAGCCTGGGACCACTTG 18 VEGF NM_003376 S4782/VEGF.p1 TTGCCTTGCTGCTCTACCTCCACCA 25 VEGFB NM_003377 S2724/VEGFB.f1 TGACGATGGCCTGGAGTGT 19 VEGFB NM_003377 S2725/VEGFB.r1 GGTACCGGATCATGAGGATCTG 22 VEGFB NM_003377 S4960/VEGFB.p1 CTGGGCAGCACCAAGTCCGGA 21 WISP1 NM_003882 S1671/WISP1.f1 AGAGGCATCCATGAACTTCACA 22 WISP1 NM_003882 S1672/WISP1.r1 CAAACTCCACAGTACTTGGGTTGA 24 WISP1 NM_003882 S4915/W1SP1.p1 CGGGCTGCATCAGCACACGC 20 XIAP NM_001167 S0289/X1AP.f1 GCAGTTGGAAGACACAGGAAAGT 23 XIAP NM_001167 S0291/XIAP.r1 TGCGTGGCACTATTTTCAAGA 21 XIAP NM_001167 S4752/XIAP.p1 TCCCCAAATTGCAGATTTATCAACGGC 27 YB-1 NM_004559 S1194/YB-1.f2 AGACTGTGGAGTTTGATGTTGTTGA 25 YB-1 NM_004559 S1195/YB-1.r2 GGAACACCACCAGGACCTGTAA 22 YB-1 NM_004559 S4843/YB-1.p2 TTGCTGCCTCCGCACCCTTTTCT 23 ZNF217 NM_006526 S2739/ZNF217.f3 ACCCAGTAGCAAGGAGAAGC 20 ZNF217 NM_006526 S2740/ZNF217.r3 CAGCTGGTGGTAGGTTCTGA 20 ZNF217 NM_006526 S4961/ZNF217.p3 CACTCACTGCTCCGAGTGCGG 21

[0217]

1 440 1 81 DNA Artificial Sequence Amplicon 1 gcggcgagtt tccgatttaa agctgagctg cgaggaaaat ggcggcggga ggatcaaaat 60 acttgctgga tggtggactc a 81 2 71 DNA Artificial Sequence Amplicon 2 cgcttctatg gcgctgagat tgtgtcagcc ctggactacc tgcactcgga gaagaacgtg 60 gtgtaccggg a 71 3 71 DNA Artificial Sequence Amplicon 3 tcctgccacc cttcaaacct caggtcacgt ccgaggtcga cacaaggtac ttcgatgatg 60 aatttaccgc c 71 4 69 DNA Artificial Sequence Amplicon 4 ggacagcagg aatgtgtttc tccatacagg tcacggggag ccaatggttc agaaacaaat 60 cgagtgggt 69 5 82 DNA Artificial Sequence Amplicon 5 tgtgagtgaa atgccttcta gtagtgaacc gtcctcggga gccgactatg actactcaga 60 agagtatgat aacgaaccac aa 82 6 66 DNA Artificial Sequence amplicon 6 cagcagatgt ggatcagcaa gcaggagtat gacgagtccg gcccctccat cgtccaccgc 60 aaatgc 66 7 80 DNA Artificial Sequence Amplicon 7 ggctcttgtg cgtactgtcc ttcgggctgg tgacagggaa gacatcactg agcctgccat 60 ctgtgctctt cgtcatctga 80 8 73 DNA Artificial Sequence Amplicon 8 gggtcaggtg cctcgagatc gggcttgggc ccagagcatg ttccagatcc cagagtttga 60 gccgagtgag cag 73 9 81 DNA Artificial Sequence Amplicon 9 cgttgtcagc acttggaata caagatggtt gccgggtcat gttaattggg aaaaagaaca 60 gtccacagga agaggttgaa c 81 10 83 DNA Artificial Sequence Amplicon 10 cctggagggt cctgtacaat ctcatcatgg gactcctgcc cttacccagg ggccacagag 60 cccccgagat ggagcccaat tag 83 11 73 DNA Artificial Sequence Amplicon 11 cagatggacc tagtacccac tgagatttcc acgccgaagg acagcgatgg gaaaaatgcc 60 cttaaatcat agg 73 12 72 DNA Artificial Sequence Amplicon 12 atcctagccc tggtttttgg cctccttttt gctgtcacca gcgtcgcgtt ccttgtgcag 60 atgagaaggc ag 72 13 84 DNA Artificial Sequence Amplicon 13 ttcaggttgt tgcaggagac catgtacatg actgtctcca ttattgatcg gttcatgcag 60 aataattgtg tgcccaagaa gatg 84 14 69 DNA Artificial Sequence Amplicon 14 gcatgttcgt ggcctctaag atgaaggaga ccatccccct gacggccgag aagctgtgca 60 tctacaccg 69 15 71 DNA Artificial Sequence Amplicon 15 aaagaagatg atgaccgggt ttacccaaac tcaacgtgca agcctcggat tattgcacca 60 tccagaggct c 71 16 82 DNA Artificial Sequence Amplicon 16 atgctgtggc tccttcctaa ctggggcttt cttgacatgt aggttgcttg gtaataacct 60 ttttgtatat cacaatttgg gt 82 17 65 DNA Artificial Sequence Amplicon 17 agatgaagtg gaaggcgctt ttcaccgcgg ccatcctgca ggcacagttg ccgattacag 60 aggca 65 18 74 DNA Artificial Sequence Amplicon 18 tggttcccag ccctgtgtcc acctccaagc ccagattcag attcgagtca tgtacacaac 60 ccagggtgga ggag 74 19 64 DNA Artificial Sequence Amplicon 19 gggcgtggaa cagtttatct cagacatctg ccccaagaag gacgtactcg aaaccttcac 60 cgtg 64 20 81 DNA Artificial Sequence Amplicon 20 tgagtgtccc ccggtatctt ccccgccctg ccaatcccga tgaaattgga aattttattg 60 atgaaaatct gaaagcggct g 81 21 77 DNA Artificial Sequence Amplicon 21 tgacaatcag cacacctgca ttcaccgctc ggaagagggc ctgagctgca tgaataagga 60 tcacggctgt agtcaca 77 22 82 DNA Artificial Sequence Amplicon 22 gataaattgg tacaagggat cagcttttcc cagcccacat gtcctgatca tatgcttttg 60 aatagtcagt tacttggcac cc 82 23 72 DNA Artificial Sequence Amplicon 23 tgcctgtggt gggaagctca gtaactggga accaaaggat gatgctatgt cagaacaccg 60 gaggcatttt cc 72 24 86 DNA Artificial Sequence Amplicon 24 ggatatttcc gtggctctta ttcaaactct ccatcaaatc ctgtaaactc cagagcaaat 60 caagattttt ctgccttgat gagaag 86 25 86 DNA Artificial Sequence Amplicon 25 gacatttcca gtcctgcagt caatgcctct ctgccccacc ctttgttcag tgtggctggt 60 gccacgacaa atgtgtgcga tcggag 86 26 75 DNA Artificial Sequence Amplicon 26 ggcatcctgg cccaaagttt cccaaatcca ggcggctaga ggcccactgc ttcccaacta 60 ccagctgagg gggtc 75 27 79 DNA Artificial Sequence Amplicon 27 tctgcagagt tggaagcact ctatggtgac atcgatgctg tggagctgta tcctgccctt 60 ctggtagaaa agcctcggc 79 28 74 DNA Artificial Sequence Amplicon 28 gggaggctta tctcactgag tgagcagaat ctggtagact gctctgggcc tcaaggcaat 60 gaaggctgca atgg 74 29 67 DNA Artificial Sequence Amplicon 29 tgtctcactg agcgagcaga atctggtgga ctgttcgcgt cctcaaggca atcagggctg 60 caatggt 67 30 77 DNA Artificial Sequence Amplicon 30 cgctgacatc atgaatgttc ctcgaccggc tggaggcgag tttggatatg acaaagacac 60 atcgttgctg aaagaga 77 31 73 DNA Artificial Sequence Amplicon 31 cacaatggcg gctctgaaga gttggctgtc gcgcagcgta acttcattct tcaggtacag 60 acagtgtttg tgt 73 32 84 DNA Artificial Sequence Amplicon 32 ctctgagaca gtgcttcgat gactttgcag acttggtgcc ctttgactcc tgggagccgc 60 tcatgaggaa gttgggcctc atgg 84 33 62 DNA Artificial Sequence Amplicon 33 tgtcgatgga cttccagaac cacctgggca gctgccaaaa gtgtgatcca agctgtccca 60 at 62 34 82 DNA Artificial Sequence Amplicon 34 gatctaagat ggcgactgtc gaaccggaaa ccacccctac tcctaatccc ccgactacag 60 aagaggagaa aacggaatct aa 82 35 68 DNA Artificial Sequence Amplicon 35 ggcagtgtca ctgagtcctt gaaatcctcc cctgccccgc gggtctctgg attgggacgc 60 acagtgca 68 36 75 DNA Artificial Sequence Amplicon 36 gggccctcca gaacaatgat gggctttatg atcctgactg cgatgagagc gggctcttta 60 aggccaagca gtgca 75 37 76 DNA Artificial Sequence Amplicon 37 accgtaggct ctgctctgaa tgactctcct gtgggtctgg ctgcctatat tctagagaag 60 ttttccacct ggacca 76 38 81 DNA Artificial Sequence Amplicon 38 cggttatgtc atgccagata cacacctcaa aggtactccc tcctcccggg aaggcaccct 60 ttcttcagtg ggtctcagtt c 81 39 68 DNA Artificial Sequence Amplicon 39 cgtggtgccc ctctatgacc tgctgctgga gatgctggac gcccaccgcc tacatgcgcc 60 cactagcc 68 40 90 DNA Artificial Sequence Amplicon 40 ggctattcct cattttctct acaaagtggc ctcagtgaac atgaagaagg tagcctcctg 60 gaggagaatt tcggtgacag tctacaatcc 90 41 68 DNA Artificial Sequence Amplicon 41 cggtagtcaa gtccggatca agggcaagga gacggaattc tacctgtgca tgaaccgcaa 60 aggcaagc 68 42 74 DNA Artificial Sequence Amplicon 42 cacgggacat tcaccacatc gactactata aaaagacaac caacggccga ctgcctgtga 60 agtggatggc accc 74 43 67 DNA Artificial Sequence Amplicon 43 ccagtggagc gcttccatga cctgcgtcct gatgaagtgg ccgatttgtt tcagacgacc 60 cagagag 67 44 75 DNA Artificial Sequence Amplicon 44 ttggtacctg tgggttagca tcaagttctc cccagggtag aattcaatca gagctccagt 60 ttgcatttgg atgtg 75 45 68 DNA Artificial Sequence Amplicon 45 tcagcagcaa gggcatcatg gaggaggatg aggcctgcgg gcgccagtac acgctcaaga 60 aaaccacc 68 46 74 DNA Artificial Sequence Amplicon 46 attccaccca tggcaaattc catggcaccg tcaaggctga gaacgggaag cttgtcatca 60 atggaaatcc catc 74 47 75 DNA Artificial Sequence Amplicon 47 caaaggagct cactgtggtg tctgtgttcc aaccactgaa tctggacccc atctgtgaat 60 aagccattct gactc 75 48 67 DNA Artificial Sequence Amplicon 48 ccatctgcat ccatcttgtt tgggctcccc acccttgaga agtgcctcag ataataccct 60 ggtggcc 67 49 73 DNA Artificial Sequence Amplicon 49 cgaaaagatg ctgaacagtg acaaatccaa ctgaccagaa gggaggagga agctcactgg 60 tggctgttcc tga 73 50 86 DNA Artificial Sequence Amplicon 50 aagctatgag gaaaagaagt acacgatggg ggacgctcct gattatgaca gaagccagtg 60 gctgaatgaa aaattcaagc tgggcc 86 51 73 DNA Artificial Sequence Amplicon 51 cccactcagt agccaagtca caatgtttgg aaaacagccc gtttacttga gcaagactga 60 taccacctgc gtg 73 52 70 DNA Artificial Sequence Amplicon 52 cggtgtgaga agtgcagcaa gccctgtgcc cgagtgtgct atggtctggg catggagcac 60 ttgcgagagg 70 53 82 DNA Artificial Sequence Amplicon 53 tgaacataaa gtctgcaaca tggaaggtat tgcactgcac aggccacatt cacgtatatg 60 ataccaacag taaccaacct ca 82 54 73 DNA Artificial Sequence Amplicon 54 tccaggatgt taggaactgt gaagatggaa gggcatgaaa ccagcgactg gaacagctac 60 tacgcagaca cgc 73 55 70 DNA Artificial Sequence Amplicon 55 agaaccgcaa ggtgagcaag gtggagattc tccagcacgt catcgactac atcagggacc 60 ttcagttgga 70 56 76 DNA Artificial Sequence Amplicon 56 tccggagctg tgatctaagg aggctggaga tgtattgcgc acccctcaag cctgccaagt 60 cagctcgctc tgtccg 76 57 83 DNA Artificial Sequence Amplicon 57 gcatggtagc cgaagatttc acagtcaaaa tcggagattt tggtatgacg cgagatatct 60 atgagacaga ctattaccgg aaa 83 58 73 DNA Artificial Sequence Amplicon 58 gtggacagca ccatgaacat gttgggcggg ggaggcagtg ctggccggaa gcccctcaag 60 tcgggtatga agg 73 59 72 DNA Artificial Sequence Amplicon 59 cctgaacctt ccaaagatgg ctgaaaaaga tggatgcttc caatctggat tcaatgagga 60 gacttgcctg gt 72 60 74 DNA Artificial Sequence Amplicon 60 ccacagctca ccttctgtca ggtgtccatc ccagctccag ccagctccca gagaggaaga 60 gactggcact gagg 74 61 80 DNA Artificial Sequence Amplicon 61 cggactttgg gtgcgacttg acgagcggtg gttcgacaag tggccttgcg ggccggatcg 60 tcccagtgga agagttgtaa 80 62 78 DNA Artificial Sequence Amplicon 62 gcccagaggc tccatcgtcc atcctcttcc tccccagtcg gctgaactct ccccttgtct 60 gcactgttca aacctctg 78 63 83 DNA Artificial Sequence Amplicon 63 ggcctgctga gatcaaagac tacagtccct acttcaagac cattgaggac ctgaggaaca 60 agattctcac agccacagtg gac 83 64 73 DNA Artificial Sequence Amplicon 64 cgaggattgg ttcttcagca agacagagga actgaaccgc gaggtggcca ccaacagtga 60 gctggtgcag agt 73 65 68 DNA Artificial Sequence Amplicon 65 agagatcgag gctctcaagg aggagctgct cttcatgaag aagaaccacg aagaggaagt 60 aaaaggcc 68 66 77 DNA Artificial Sequence Amplicon 66 tgagcggcag aatcaggagt accagcggct catggacatc aagtcgcggc tggagcagga 60 gattgccacc taccgca 77 67 69 DNA Artificial Sequence Amplicon 67 tcagtggaga aggagttgga ccagtcaaca tctctgttgt cacaagcagt gtttcctctg 60 gatatggca 69 68 86 DNA Artificial Sequence Amplicon 68 ggatgaagct tacatgaaca aggtagagct ggagtctcgc ctggaagggc tgaccgacga 60 gatcaacttc ctcaggcagc tatatg 86 69 83 DNA Artificial Sequence Amplicon 69 ggaaagacca cctgaaaaac cacctccaga cccacgaccc caacaaaatg gcctttgggt 60 gtgaggagtg tgggaagaag tac 83 70 77 DNA Artificial Sequence Amplicon 70 cagatggcca ctttgagaac attttagctg acaacagtgt gaacgaccag accaaaatcc 60 ttgtggttaa tgctgcc 77 71 75 DNA Artificial Sequence Amplicon 71 gacttttgcc cgctaccttt cattccggcg tgacaacaat gagctgttgc tcttcatact 60 gaagcagtta gtggc 75 72 75 DNA Artificial Sequence Amplicon 72 ggagaacaat ccccttgaga cagaatatgg cctttctgtc tacaaggatc accagaccat 60 caccatccag gagat 75 73 82 DNA Artificial Sequence Amplicon 73 tgatggtcct atgtgtcaca ttcatcacag gtttcatacc aacacaggct tcagcacttc 60 ctttggtgtg tttcctgtcc ca 82 74 68 DNA Artificial Sequence Amplicon 74 ctacagggac gccatcgaat ccggatcttg atgctggtgt aagtgaacat tcaggtgatt 60 ggttggat 68 75 67 DNA Artificial Sequence Amplicon 75 gagaaccaat ctcaccgaca ggcagctggc agaggaatac ctgtaccgct atggttacac 60 tcgggtg 67 76 77 DNA Artificial Sequence Amplicon 76 ccgccctcac ctgaagagaa acgcgctcct tggcggacac tgggggagga gaggaagaag 60 cgcggctaac ttattcc 77 77 74 DNA Artificial Sequence Amplicon 77 gccgagatcg ccaagatgtt gccagggagg acagacaatg ctgtgaagaa tcactggaac 60 tctaccatca aaag 74 78 72 DNA Artificial Sequence Amplicon 78 ccctcgtgct gatgctactg aggagccagc gtctagggca gcagccgctt cctagaagac 60 caggtcatga tg 72 79 66 DNA Artificial Sequence Amplicon 79 cggtggacca cgaagagtta acccgggact tggagaagca ctgcagagac atggaagagg 60 cgagcc 66 80 68 DNA Artificial Sequence Amplicon 80 ctttgaaccc ttgcttgcaa taggtgtgcg tcagaagcac ccaggacttc catttgcttt 60 gtcccggg 68 81 81 DNA Artificial Sequence Amplicon 81 ccgcaacgtg gttttctcac cctatggggt ggcctcggtg ttggccatgc tccagctgac 60 aacaggagga gaaacccagc a 81 82 66 DNA Artificial Sequence Amplicon 82 ccagctctcc ttccagctac agatcaatgt ccctgtccga gtgctggagc taagtgagag 60 ccaccc 66 83 83 DNA Artificial Sequence Amplicon 83 ataccaatca ccgcacaaac ccaggctatt tgttaagtcc agtcacagcg caaagaaaca 60 tatgcggaga aaatgctagt gtg 83 84 62 DNA Artificial Sequence Amplicon 84 gccatccgca aaggctttct cgcttgtcac cttgccatgt ggaagaaact ggcggaatgg 60 cc 62 85 85 DNA Artificial Sequence Amplicon 85 gcatcaggct gtcattatgg tgtccttacc tgtgggagct gtaaggtctt ctttaagagg 60 gcaatggaag ggcagcacaa ctact 85 86 66 DNA Artificial Sequence Amplicon 86 tctccatatc tgccttgcag agtctcctgc agcacctcat cgggctgagc aatctgaccc 60 acgtgc 66 87 86 DNA Artificial Sequence Amplicon 87 gccctcccag tgtgcaaata agggctgctg tttcgacgac accgttcgtg gggtcccctg 60 gtgcttctat cctaatacca tcgacg 86 88 78 DNA Artificial Sequence Amplicon 88 gaacttcttg agcaggagca tacccagggc ttcataatca ccttctgttc agcactagat 60 gatattcttg ggggtgga 78 89 77 DNA Artificial Sequence Amplicon 89 cgaagccctt acaagtttcc tagttcaccc ttacggattc ctggagggaa catctatatt 60 tcacccctga agagtcc 77 90 74 DNA Artificial Sequence Amplicon 90 ccagacgagc gattagaagc ggcagcttgt gaggtgaatg atttggggga agaggaggag 60 gaggaagagg agga 74 91 69 DNA Artificial Sequence Amplicon 91 catcttccag gaggaccact ctctgtggca ccctggacta cctgccccct gaaatgattg 60 aaggtcgga 69 92 90 DNA Artificial Sequence Amplicon 92 cctggaggct gcaacatacc tcaatcctgt cccaggccgg atcctcctga agcccttttc 60 gcagcactgc tatcctccaa agccattgta 90 93 80 DNA Artificial Sequence Amplicon 93 tgttttgatt cccgggctta ccaggtgaga agtgagggag gaagaaggca gtgtcccttt 60 tgctagagct gacagctttg 80 94 65 DNA Artificial Sequence Amplicon 94 gcccgaaacg ccgaatataa tcccaagcgg tttgctgcgg taatcatgag gataagagag 60 ccacg 65 95 83 DNA Artificial Sequence Amplicon 95 ggtgtgccac agaccttcct acttggcctg taatcacctg tgcagccttt tgtgggcctt 60 caaaactctg tcaagaactc cgt 83 96 75 DNA Artificial Sequence Amplicon 96 tccctgcggt cccagatagc ctgaatcctg cccggagtgg aactgaagcc tgcacagtgt 60 ccaccctgtt cccac 75 97 72 DNA Artificial Sequence Amplicon 97 aatccaaggg ggagagtgat gacttccata tggactttga ctcagctgtg gctcctcggg 60 caaaatctgt ac 72 98 66 DNA Artificial Sequence Amplicon 98 tgtggacatc ttcccctcag acttccctac tgagccacct tctctgccac gaaccggtcg 60 ggctag 66 99 82 DNA Artificial Sequence Amplicon 99 ctatatgcag ccagagatgt gacagccacc gtggacagcc tgccactcat cacagcctcc 60 attctcagta agaaactcgt gg 82 100 81 DNA Artificial Sequence Amplicon 100 gggccaaata ttcagaagct tttatatcag aggaccacca tagcggccat ggagaccatc 60 tctgtcccat catacccatc c 81 101 73 DNA Artificial Sequence Amplicon 101 cttcacagtg ctcctgcagt ctctctgtgt ggctgtaact tacgtgtact ttaccaacga 60 gctgaagcag atg 73 102 65 DNA Artificial Sequence Amplicon 102 gcctcggtgt gcctttcaac atcgccagct acgccctgct cacgtacatg attgcgcaca 60 tcacg 65 103 70 DNA Artificial Sequence Amplicon 103 gtggatgtgc cctgaaggac aagccaggcg tctacacgag agtctcacac ttcttaccct 60 ggatccgcag 70 104 67 DNA Artificial Sequence Amplicon 104 gccctggatt tcagaaagag ccaagtctgg atctgggacc ctttccttcc ttccctggct 60 tgtaact 67 105 71 DNA Artificial Sequence Amplicon 105 ctgctgtctt gggtgcattg gagccttgcc ttgctgctct acctccacca tgccaagtgg 60 tcccaggctg c 71 106 71 DNA Artificial Sequence Amplicon 106 tgacgatggc ctggagtgtg tgcccactgg gcagcaccaa gtccggatgc agatcctcat 60 gatccggtac c 71 107 75 DNA Artificial Sequence Amplicon 107 agaggcatcc atgaacttca cacttgcggg ctgcatcagc acacgctcct atcaacccaa 60 gtactgtgga gtttg 75 108 77 DNA Artificial Sequence Amplicon 108 gcagttggaa gacacaggaa agtatcccca aattgcagat ttatcaacgg cttttatctt 60 gaaaatagtg ccacgca 77 109 76 DNA Artificial Sequence Amplicon 109 agactgtgga gtttgatgtt gttgaaggag aaaagggtgc ggaggcagca aatgttacag 60 gtcctggtgg tgttcc 76 110 70 DNA Artificial Sequence Amplicon 110 acccagtagc aaggagaagc ccactcactg ctccgagtgc ggcaaagctt tcagaaccta 60 ccaccagctg 70 111 19 DNA Artificial Sequence forward primer 111 gcggcgagtt tccgattta 19 112 21 DNA Artificial Sequence reverse primer 112 tgagtccacc atccagcaag t 21 113 21 DNA Artificial Sequence probe 113 atggcggcgg gaggatcaaa a 21 114 20 DNA Artificial Sequence forward primer 114 cgcttctatg gcgctgagat 20 115 20 DNA Artificial Sequence reverse primer 115 tcccggtaca ccacgttctt 20 116 24 DNA Artificial Sequence probe 116 cagccctgga ctacctgcac tcgg 24 117 19 DNA Artificial Sequence forward primer 117 tcctgccacc cttcaaacc 19 118 21 DNA Artificial Sequence reverse primer 118 ggcggtaaat tcatcatcga a 21 119 24 DNA Artificial Sequence probe 119 caggtcacgt ccgaggtcga caca 24 120 20 DNA Artificial Sequence forward primer 120 ggacagcagg aatgtgtttc 20 121 20 DNA Artificial Sequence reverse primer 121 acccactcga tttgtttctg 20 122 22 DNA Artificial Sequence probe 122 cattggctcc ccgtgacctg ta 22 123 27 DNA Artificial Sequence forward primer 123 tgtgagtgaa atgccttcta gtagtga 27 124 23 DNA Artificial Sequence probe 124 ccgtcctcgg gagccgacta tga 23 125 27 DNA Artificial Sequence reverse primer 125 ttgtggttcg ttatcatact cttctga 27 126 21 DNA Artificial Sequence forward primer 126 cagcagatgt ggatcagcaa g 21 127 18 DNA Artificial Sequence reverse primer 127 gcatttgcgg tggacgat 18 128 23 DNA Artificial Sequence probe 128 aggagtatga cgagtccggc ccc 23 129 22 DNA Artificial Sequence forward primer 129 ggctcttgtg cgtactgtcc tt 22 130 23 DNA Artificial Sequence reverse primer 130 tcagatgacg aagagcacag atg 23 131 29 DNA Artificial Sequence probe 131 aggctcagtg atgtcttccc tgtcaccag 29 132 19 DNA Artificial Sequence forward primer 132 gggtcaggtg cctcgagat 19 133 21 DNA Artificial Sequence reverse primer 133 ctgctcactc ggctcaaact c 21 134 24 DNA Artificial Sequence probe 134 tgggcccaga gcatgttcca gatc 24 135 23 DNA Artificial Sequence forward primer 135 cgttgtcagc acttggaata caa 23 136 24 DNA Artificial Sequence reverse primer 136 gttcaacctc ttcctgtgga ctgt 24 137 26 DNA Artificial Sequence probe 137 cccaattaac atgacccggc aaccat 26 138 20 DNA Artificial Sequence forward primer 138 cctggagggt cctgtacaat 20 139 19 DNA Artificial Sequence reverse primer 139 ctaattgggc tccatctcg 19 140 24 DNA Artificial Sequence probe 140 catcatggga ctcctgccct tacc 24 141 25 DNA Artificial Sequence forward primer 141 cagatggacc tagtacccac tgaga 25 142 22 DNA Artificial Sequence probe 142 ttccacgccg aaggacagcg at 22 143 24 DNA Artificial Sequence reverse primer 143 cctatgattt aagggcattt ttcc 24 144 20 DNA Artificial Sequence forward primer 144 atcctagccc tggtttttgg 20 145 20 DNA Artificial sequence reverse primer 145 ctgccttctc atctgcacaa 20 146 20 DNA Artificial Sequence probe 146 tttgctgtca ccagcgtcgc 20 147 20 DNA Artificial Sequence forward primer 147 ttcaggttgt tgcaggagac 20 148 20 DNA Artificial Sequence reverse primer 148 catcttcttg ggcacacaat 20 149 27 DNA Artificial Sequence probe 149 tgtctccatt attgatcggt tcatgca 27 150 21 DNA Artificial Sequence forward primer 150 gcatgttcgt ggcctctaag a 21 151 22 DNA Artificial Sequence reverse primer 151 cggtgtagat gcacagcttc tc 22 152 23 DNA Artificial Sequence probe 152 aaggagacca tccccctgac ggc 23 153 24 DNA Artificial Sequence forward primer 153 aaagaagatg atgaccgggt ttac 24 154 20 DNA Artificial Sequence reverse primer 154 gagcctctgg atggtgcaat 20 155 24 DNA Artificial Sequence probe 155 caaactcaac gtgcaagcct cgga 24 156 22 DNA Artificial Sequence forward primer 156 atgctgtggc tccttcctaa ct 22 157 27 DNA Artificial Sequence reverse primer 157 acccaaattg tgatatacaa aaaggtt 27 158 30 DNA Artificial Sequence probe 158 taccaagcaa cctacatgtc aagaaagccc 30 159 20 DNA Artificial Sequence forward primer 159 agatgaagtg gaaggcgctt 20 160 18 DNA Artificial Sequence probe 160 caccgcggcc atcctgca 18 161 21 DNA Artificial Sequence reverse primer 161 tgcctctgta atcggcaact g 21 162 18 DNA Artificial Sequence forward primer 162 tggttcccag ccctgtgt 18 163 28 DNA Artificial Sequence probe 163 ctccaagccc agattcagat tcgagtca 28 164 19 DNA Artificial Sequence reverse primer 164 ctcctccacc ctgggttgt 19 165 20 DNA Artificial Sequence forward primer 165 gggcgtggaa cagtttatct 20 166 19 DNA Artificial Sequence reverse primer 166 cacggtgaag gtttcgagt 19 167 24 DNA Artificial Sequence probe 167 agacatctgc cccaagaagg acgt 24 168 21 DNA Artificial Sequence forward primer 168 tgagtgtccc ccggtatctt c 21 169 21 DNA Artificial Sequence reverse primer 169 cagccgcttt cagattttca t 21 170 27 DNA Artificial Sequence probe 170 tgccaatccc gatgaaattg gaaattt 27 171 21 DNA Artificial Sequence forward primer 171 tgacaatcag cacacctgca t 21 172 23 DNA Artificial Sequence reverse primer 172 tgtgactaca gccgtgatcc tta 23 173 20 DNA Artificial Sequence probe 173 caggccctct tccgagcggt 20 174 26 DNA Artificial Sequence forward primer 174 gataaattgg tacaagggat cagctt 26 175 24 DNA Artificial Sequence reverse primer 175 gggtgccaag taactgacta ttca 24 176 26 DNA Artificial Sequence probe 176 ccagcccaca tgtcctgatc atatgc 26 177 18 DNA Artificial Sequence forward primer 177 tgcctgtggt gggaagct 18 178 19 DNA Artificial Sequence reverse primer 178 ggaaaatgcc tccggtgtt 19 179 30 DNA Artificial Sequence probe 179 tgacatagca tcatcctttg gttcccagtt 30 180 24 DNA Artificial Sequence forward primer 180 ggatatttcc gtggctctta ttca 24 181 30 DNA Artificial Sequence probe 181 tctccatcaa atcctgtaaa ctccagagca 30 182 25 DNA Artificial Sequence reverse primer 182 cttctcatca aggcagaaaa atctt 25 183 22 DNA Artificial Sequence forward primer 183 gacatttcca gtcctgcagt ca 22 184 23 DNA Artificial Sequence probe 184 tgcctctctg ccccaccctt tgt 23 185 20 DNA Artificial Sequence reverse primer 185 ctccgatcgc acacatttgt 20 186 18 DNA Artificial Sequence forward primer 186 ggcatcctgg cccaaagt 18 187 21 DNA Artificial Sequence reverse primer 187 gaccccctca gctggtagtt g 21 188 23 DNA Artificial Sequence probe 188 cccaaatcca ggcggctaga ggc 23 189 23 DNA Artificial Sequence forward primer 189 tctgcagagt tggaagcact cta 23 190 28 DNA Artificial Sequence probe 190 caggatacag ctccacagca tcgatgtc 28 191 21 DNA Artificial Sequence reverse primer 191 gccgaggctt ttctaccaga a 21 192 23 DNA Artificial Sequence forward primer 192 gggaggctta tctcactgag tga 23 193 19 DNA Artificial Sequence reverse primer 193 ccattgcagc cttcattgc 19 194 29 DNA Artificial Sequence probe 194 ttgaggccca gagcagtcta ccagattct 29 195 21 DNA Artificial Sequence forward primer 195 tgtctcactg agcgagcaga a 21 196 19 DNA Artificial Sequence reverse primer 196 accattgcag ccctgattg 19 197 24 DNA Artificial Sequence probe 197 cttgaggacg cgaacagtcc acca 24 198 22 DNA Artificial Sequence forward primer 198 cgctgacatc atgaatgttc ct 22 199 24 DNA Artificial Sequence reverse primer 199 tctctttcag caacgatgtg tctt 24 200 25 DNA Artificial Sequence probe 200 tcatatccaa actcgcctcc agccg 25 201 19 DNA Artificial Sequence forward primer 201 cacaatggcg gctctgaag 19 202 26 DNA Artificial Sequence reverse primer 202 acacaaacac tgtctgtacc tgaaga 26 203 23 DNA Artificial Sequence probe 203 aagttacgct gcgcgacagc caa 23 204 24 DNA Artificial Sequence forward primer 204 ctctgagaca gtgcttcgat gact 24 205 19 DNA Artificial Sequence reverse primer 205 ccatgaggcc caacttcct 19 206 23 DNA Artificial Sequence probe 206 cagacttggt gccctttgac tcc 23 207 20 DNA Artificial Sequence forward primer 207 tgtcgatgga cttccagaac 20 208 18 DNA Artificial Sequence probe 208 cacctgggca gctgccaa 18 209 19 DNA Artificial Sequence reverse primer 209 attgggacag cttggatca 19 210 23 DNA Artificial Sequence forward primer 210 gatctaagat ggcgactgtc gaa 23 211 25 DNA Artificial Sequence reverse primer 211 ttagattccg ttttctcctc ttctg 25 212 27 DNA Artificial Sequence probe 212 accaccccta ctcctaatcc cccgact 27 213 22 DNA Artificial Sequence forward primer 213 ggcagtgtca ctgagtcctt ga 22 214 18 DNA Artificial Sequence reverse primer 214 tgcactgtgc gtcccaat 18 215 18 DNA Artificial Sequence probe 215 atcctcccct gccccgcg 18 216 20 DNA Artificial Sequence forward primer 216 gggccctcca gaacaatgat 20 217 21 DNA Artificial Sequence reverse primer 217 tgcactgctt ggccttaaag a 21 218 25 DNA Artificial Sequence probe 218 ccgctctcat cgcagtcagg atcat 25 219 20 DNA Artificial Sequence forward primer 219 accgtaggct ctgctctgaa 20 220 20 DNA Artificial Sequence reverse primer 220 tggtccaggt ggaaaacttc 20 221 20 DNA Artificial Sequence probe 221 aggcagccag acccacagga 20 222 23 DNA Artificial Sequence forward primer 222 cggttatgtc atgccagata cac 23 223 25 DNA Artificial Sequence probe 223 cctcaaaggt actccctcct cccgg 25 224 24 DNA Artificial Sequence reverse primer 224 gaactgagac ccactgaaga aagg 24 225 19 DNA Artificial Sequence forward primer 225 cgtggtgccc ctctatgac 19 226 19 DNA Artificial Sequence probe 226 ctggagatgc tggacgccc 19 227 19 DNA Artificial Sequence reverse primer 227 ggctagtggg cgcatgtag 19 228 25 DNA Artificial Sequence reverse primer 228 ggattgtaga ctgtcaccga aattc 25 229 28 DNA Artificial Sequence forward primer 229 ggctattcct cattttctct acaaagtg 28 230 30 DNA Artificial Sequence probe 230 cctccaggag gctaccttct tcatgttcac 30 231 21 DNA Artificial Sequence forward primer 231 cggtagtcaa gtccggatca a 21 232 18 DNA Artificial Sequence reverse primer 232 gcttgccttt gcggttca 18 233 25 DNA Artificial Sequence probe 233 caaggagacg gaattctacc tgtgc 25 234 20 DNA Artificial Sequence forward primer 234 cacgggacat tcaccacatc 20 235 19 DNA Artificial Sequence reverse primer 235 gggtgccatc cacttcaca 19 236 27 DNA Artificial Sequence probe 236 ataaaaagac aaccaacggc cgactgc 27 237 18 DNA Artificial Sequence forward primer 237 ccagtggagc gcttccat 18 238 22 DNA Artificial Sequence reverse primer 238 ctctctgggt cgtctgaaac aa 22 239 23 DNA Artificial Sequence probe 239 tcggccactt catcaggacg cag 23 240 20 DNA Artificial Sequence forward primer 240 ttggtacctg tgggttagca 20 241 20 DNA Artificial Sequence reverse primer 241 cacatccaaa tgcaaactgg 20 242 26 DNA Artificial Sequence probe 242 tccccagggt agaattcaat cagagc 26 243 19 DNA Artificial Sequence forward primer 243 tcagcagcaa gggcatcat 19 244 23 DNA Artificial Sequence reverse primer 244 ggtggttttc ttgagcgtgt act 23 245 19 DNA Artificial Sequence probe 245 cgcccgcagg cctcatcct 19 246 20 DNA Artificial Sequence forward primer 246 attccaccca tggcaaattc 20 247 22 DNA Artificial Sequence reverse primer 247 gatgggattt ccattgatga ca 22 248 22 DNA Artificial Sequence probe 248 ccgttctcag ccttgacggt gc 22 249 23 DNA Artificial Sequence forward primer 249 caaaggagct cactgtggtg tct 23 250 24 DNA Artificial Sequence probe 250 tgttccaacc actgaatctg gacc 24 251 26 DNA Artificial Sequence reverse primer 251 gagtcagaat ggcttattca cagatg 26 252 20 DNA Artificial Sequence forward primer 252 ccatctgcat ccatcttgtt 20 253 23 DNA Artificial Sequence probe 253 ctccccaccc ttgagaagtg cct 23 254 20 DNA Artificial Sequence reverse primer 254 ggccaccagg gtattatctg 20 255 23 DNA Artificial Sequence forward primer 255 cgaaaagatg ctgaacagtg aca 23 256 20 DNA Artificial Sequence reverse primer 256 tcaggaacag ccaccagtga 20 257 28 DNA Artificial Sequence probe 257 cttcctcctc ccttctggtc agttggat 28 258 20 DNA Artificial Sequence reverse primer 258 ggcccagctt gaatttttca 20 259 27 DNA Artificial Sequence forward primer 259 aagctatgag gaaaagaagt acacgat 27 260 30 DNA Artificial Sequence probe 260 tcagccactg gcttctgtca taatcaggag 30 261 20 DNA Artificial Sequence forward primer 261 cccactcagt agccaagtca 20 262 27 DNA Artificial Sequence probe 262 tcaagtaaac gggctgtttt ccaaaca 27 263 20 DNA Artificial Sequence reverse primer 263 cacgcaggtg gtatcagtct 20 264 20 DNA Artificial Sequence forward primer 264 cggtgtgaga agtgcagcaa 20 265 24 DNA Artificial Sequence probe 265 ccagaccata gcacactcgg gcac 24 266 19 DNA Artificial Sequence reverse primer 266 cctctcgcaa gtgctccat 19 267 24 DNA Artificial Sequence forward primer 267 tgaacataaa gtctgcaaca tgga 24 268 28 DNA Artificial Sequence reverse primer 268 tgaggttggt tactgttggt atcatata 28 269 24 DNA Artificial Sequence probe 269 ttgcactgca caggccacat tcac 24 270 24 DNA Artificial Sequence forward primer 270 tccaggatgt taggaactgt gaag 24 271 22 DNA Artificial Sequence reverse primer 271 gcgtgtctgc gtagtagctg tt 22 272 24 DNA Artificial Sequence probe 272 agtcgctggt ttcatgccct tcca 24 273 19 DNA Artificial Sequence forward primer 273 agaaccgcaa ggtgagcaa 19 274 21 DNA Artificial Sequence reverse primer 274 tccaactgaa ggtccctgat g 21 275 26 DNA Artificial Sequence probe 275 tggagattct ccagcacgtc atcgac 26 276 21 DNA Artificial Sequence forward primer 276 tccggagctg tgatctaagg a 21 277 24 DNA Artificial Sequence probe 277 tgtattgcgc acccctcaag cctg 24 278 20 DNA Artificial Sequence reverse primer 278 cggacagagc gagctgactt 20 279 21 DNA Artificial Sequence forward primer 279 gcatggtagc cgaagatttc a 21 280 30 DNA Artificial Sequence reverse primer 280 tttccggtaa tagtctgtct catagatatc 30 281 28 DNA Artificial Sequence probe 281 cgcgtcatac caaaatctcc gattttga 28 282 19 DNA Artificial Sequence forward primer 282 gtggacagca ccatgaaca 19 283 20 DNA Artificial Sequence reverse primer 283 ccttcatacc cgacttgagg 20 284 20 DNA Artificial Sequence probe 284 cttccggcca gcactgcctc 20 285 20 DNA Artificial Sequence forward primer 285 cctgaacctt ccaaagatgg 20 286 20 DNA Artificial Sequence reverse primer 286 accaggcaag tctcctcatt 20 287 27 DNA Artificial Sequence probe 287 ccagattgga agcatccatc tttttca 27 288 20 DNA Artificial Sequence forward primer 288 ccacagctca ccttctgtca 20 289 20 DNA Artificial Sequence reverse primer 289 cctcagtgcc agtctcttcc 20 290 20 DNA Artificial Sequence probe 290 tccatcccag ctccagccag 20 291 23 DNA Artificial Sequence probe 291 ccacttgtcg aaccaccgct cgt 23 292 19 DNA Artificial Sequence forward primer 292 cggactttgg gtgcgactt 19 293 24 DNA Artificial Sequence reverse primer 293 ttacaactct tccactggga cgat 24 294 18 DNA Artificial Sequence forward primer 294 gcccagaggc tccatcgt 18 295 23 DNA Artificial Sequence reverse primer 295 cagaggtttg aacagtgcag aca 23 296 23 DNA Artificial Sequence probe 296 cctcttcctc cccagtcggc tga 23 297 20 DNA Artificial Sequence forward primer 297 ggcctgctga gatcaaagac 20 298 20 DNA Artificial Sequence reverse primer 298 gtccactgtg gctgtgagaa 20 299 26 DNA Artificial Sequence probe 299 tgttcctcag gtcctcaatg gtcttg 26 300 21 DNA Artificial Sequence forward primer 300 cgaggattgg ttcttcagca a 21 301 22 DNA Artificial Sequence reverse primer 301 actctgcacc agctcactgt tg 22 302 24 DNA Artificial Sequence probe 302 cacctcgcgg ttcagttcct ctgt 24 303 20 DNA Artificial Sequence forward primer 303 agagatcgag gctctcaagg 20 304 20 DNA Artificial Sequence reverse primer 304 ggccttttac ttcctcttcg 20 305 27 DNA Artificial Sequence probe 305 tggttcttct tcatgaagag cagctcc 27 306 21 DNA Artificial Sequence forward primer 306 tgagcggcag aatcaggagt a 21 307 19 DNA Artificial Sequence reverse primer 307 tgcggtaggt ggcaatctc 19 308 24 DNA Artificial Sequence probe 308 ctcatggaca tcaagtcgcg gctg 24 309 20 DNA Artificial Sequence forward primer 309 tcagtggaga aggagttgga 20 310 28 DNA Artificial Sequence probe 310 ccagtcaaca tctctgttgt cacaagca 28 311 20 DNA Artificial Sequence reverse primer 311 tgccatatcc agaggaaaca 20 312 27 DNA Artificial Sequence forward primer 312 ggatgaagct tacatgaaca aggtaga 27 313 25 DNA Artificial Sequence reverse primer 313 catatagctg cctgaggaag ttgat 25 314 21 DNA Artificial Sequence probe 314 cgtcggtcag cccttccagg c 21 315 22 DNA Artificial Sequence forward primer 315 ggaaagacca cctgaaaaac ca 22 316 24 DNA Artificial Sequence reverse primer 316 gtacttcttc ccacactcct caca 24 317 23 DNA Artificial Sequence probe 317 acccacgacc ccaacaaaat ggc 23 318 23 DNA Artificial Sequence forward primer 318 cagatggcca ctttgagaac att 23 319 22 DNA Artificial Sequence reverse primer 319 ggcagcatta accacaagga tt 22 320 28 DNA Artificial Sequence probe 320 agctgacaac agtgtgaacg accagacc 28 321 21 DNA Artificial Sequence forward primer 321 gacttttgcc cgctaccttt c 21 322 26 DNA Artificial Sequence reverse primer 322 gccactaact gcttcagtat gaagag 26 323 24 DNA Artificial Sequence probe 323 acagctcatt gttgtcacgc cgga 24 324 20 DNA Artificial Sequence forward primer 324 ggagaacaat ccccttgaga 20 325 20 DNA Artificial Sequence reverse primer 325 atctcctgga tggtgatggt 20 326 27 DNA Artificial Sequence probe 326 tggcctttct gtctacaagg atcacca 27 327 24 DNA Artificial Sequence forward primer 327 tgatggtcct atgtgtcaca ttca 24 328 20 DNA Artificial Sequence reverse primer 328 tgggacagga aacacaccaa 20 329 30 DNA Artificial Sequence probe 329 caggtttcat accaacacag gcttcagcac 30 330 19 DNA Artificial Sequence forward primer 330 ctacagggac gccatcgaa 19 331 23 DNA Artificial Sequence reverse primer 331 atccaaccaa tcacctgaat gtt 23 332 23 DNA Artificial Sequence probe 332 cttacaccag catcaagatc cgg 23 333 20 DNA Artificial Sequence forward primer 333 gagaaccaat ctcaccgaca 20 334 20 DNA Artificial Sequence reverse primer 334 cacccgagtg taaccatagc 20 335 24 DNA Artificial Sequence probe 335 acaggtattc ctctgccagc tgcc 24 336 19 DNA Artificial Sequence forward primer 336 ccgccctcac ctgaagaga 19 337 22 DNA Artificial Sequence reverse primer 337 ggaataagtt agccgcgctt ct 22 338 21 DNA Artificial Sequence probe 338 cccagtgtcc gccaaggagc g 21 339 18 DNA Artificial Sequence forward primer 339 gccgagatcg ccaagatg 18 340 27 DNA Artificial Sequence reverse primer 340 cttttgatgg tagagttcca gtgattc 27 341 24 DNA Artificial Sequence probe 341 cagcattgtc tgtcctccct ggca 24 342 19 DNA Artificial Sequence forward primer 342 ccctcgtgct gatgctact 19 343 22 DNA Artificial Sequence reverse primer 343 catcatgacc tggtcttcta gg 22 344 22 DNA Artificial Sequence probe 344 ctgccctaga cgctggctcc tc 22 345 21 DNA Artificial Sequence forward primer 345 cggtggacca cgaagagtta a 21 346 23 DNA Artificial Sequence probe 346 ccgggacttg gagaagcact gca 23 347 19 DNA Artificial Sequence reverse primer 347 ggctcgcctc ttccatgtc 19 348 20 DNA Artificial Sequence forward primer 348 ctttgaaccc ttgcttgcaa 20 349 25 DNA Artificial Sequence probe 349 aagtcctggg tgcttctgac gcaca 25 350 18 DNA Artificial Sequence reverse primer 350 cccgggacaa agcaaatg 18 351 19 DNA Artificial Sequence forward primer 351 ccgcaacgtg gttttctca 19 352 22 DNA Artificial Sequence probe 352 ctcggtgttg gccatgctcc ag 22 353 21 DNA Artificial Sequence reverse primer 353 tgctgggttt ctcctcctgt t 21 354 20 DNA Artificial Sequence forward primer 354 ccagctctcc ttccagctac 20 355 20 DNA Artificial Sequence reverse primer 355 gggtggctct cacttagctc 20 356 24 DNA Artificial Sequence probe 356 atcaatgtcc ctgtccgagt gctg 24 357 23 DNA Artificial Sequence reverse primer 357 cacactagca ttttctccgc ata 23 358 21 DNA Artificial Sequence forward primer 358 ataccaatca ccgcacaaac c 21 359 30 DNA Artificial Sequence probe 359 tgcgctgtga ctggacttaa caaatagcct 30 360 18 DNA Artificial Sequence forward primer 360 gccatccgca aaggcttt 18 361 18 DNA Artificial Sequence reverse primer 361 ggccattccg ccagtttc 18 362 23 DNA Artificial Sequence probe 362 tcgcttgtca ccttgccatg tgg 23 363 20 DNA Artificial Sequence forward primer 363 gcatcaggct gtcattatgg 20 364 20 DNA Artificial Sequence reverse primer 364 agtagttgtg ctgcccttcc 20 365 28 DNA Artificial Sequence probe 365 tgtccttacc tgtgggagct gtaaggtc 28 366 23 DNA Artificial Sequence forward primer 366 tctccatatc tgccttgcag agt 23 367 19 DNA Artificial Sequence reverse primer 367 gcacgtgggt cagattgct 19 368 22 DNA Artificial Sequence probe 368 tcctgcagca cctcatcggg ct 22 369 19 DNA Artificial Sequence forward primer 369 gccctcccag tgtgcaaat 19 370 23 DNA Artificial Sequence probe 370 tgctgtttcg acgacaccgt tcg 23 371 25 DNA Artificial Sequence reverse primer 371 cgtcgatggt attaggatag aagca 25 372 24 DNA Artificial Sequence forward primer 372 gaacttcttg agcaggagca tacc 24 373 25 DNA Artificial Sequence reverse primer 373 tccaccccca agaatatcat ctagt 25 374 25 DNA Artificial Sequence probe 374 agggcttcat aatcaccttc tgttc 25 375 20 DNA Artificial Sequence forward primer 375 cgaagccctt acaagtttcc 20 376 20 DNA Artificial Sequence reverse primer 376 ggactcttca ggggtgaaat 20 377 24 DNA Artificial Sequence probe 377 cccttacgga ttcctggagg gaac 24 378 20 DNA Artificial Sequence forward primer 378 ccagacgagc gattagaagc 20 379 20 DNA Artificial Sequence reverse primer 379 tcctcctctt cctcctcctc 20 380 23 DNA Artificial Sequence probe 380 tgtgaggtga atgatttggg gga 23 381 20 DNA Artificial Sequence forward primer 381 catcttccag gaggaccact 20 382 20 DNA Artificial Sequence reverse primer 382 tccgaccttc aatcatttca 20 383 24 DNA Artificial Sequence probe 383 ctctgtggca ccctggacta cctg 24 384 20 DNA Artificial Sequence forward primer 384 cctggaggct gcaacatacc 20 385 23 DNA Artificial Sequence reverse primer 385 tacaatggct ttggaggata gca 23 386 25 DNA Artificial Sequence probe 386 atcctcctga agcccttttc gcagc 25 387 20 DNA Artificial Sequence forward primer 387 tgttttgatt cccgggctta 20 388 28 DNA Artificial Sequence probe 388 tgccttcttc ctccctcact tctcacct 28 389 24 DNA Artificial Sequence reverse primer 389 caaagctgtc agctctagca aaag 24 390 19 DNA Artificial Sequence forward primer 390 gcccgaaacg ccgaatata 19 391 21 DNA Artificial Sequence probe 391 taccgcagca aaccgcttgg g 21 392 23 DNA Artificial Sequence reverse primer 392 cgtggctctc ttatcctcat gat 23 393 20 DNA Artificial Sequence forward primer 393 ggtgtgccac agaccttcct 20 394 24 DNA Artificial Sequence reverse primer 394 acggagttct tgacagagtt ttga 24 395 27 DNA Artificial Sequence probe 395 ttggcctgta atcacctgtg cagcctt 27 396 19 DNA Artificial Sequence forward primer 396 tccctgcggt cccagatag 19 397 20 DNA Artificial Sequence reverse primer 397 gtgggaacag ggtggacact 20 398 25 DNA Artificial Sequence probe 398 atcctgcccg gagtggaact gaagc 25 399 20 DNA Artificial Sequence forward primer 399 aatccaaggg ggagagtgat 20 400 26 DNA Artificial Sequence probe 400 catatggact ttgactcagc tgtggc 26 401 20 DNA Artificial Sequence reverse primer 401 gtacagattt tgcccgagga 20 402 21 DNA Artificial Sequence forward primer 402 tgtggacatc ttcccctcag a 21 403 24 DNA Artificial Sequence probe 403 ttccctactg agccaccttc tctg 24 404 18 DNA Artificial Sequence reverse primer 404 ctagcccgac cggttcgt 18 405 24 DNA Artificial Sequence forward primer 405 ctatatgcag ccagagatgt gaca 24 406 23 DNA Artificial Sequence probe 406 acagcctgcc actcatcaca gcc 23 407 24 DNA Artificial Sequence reverse primer 407 ccacgagttt cttactgaga atgg 24 408 19 DNA Artificial Sequence forward primer 408 gggccaaata ttcagaagc 19 409 20 DNA Artificial Sequence reverse primer 409 ggatgggtat gatgggacag 20 410 20 DNA Artificial Sequence probe 410 ccaccatagc ggccatggag 20 411 22 DNA Artificial Sequence forward primer 411 cttcacagtg ctcctgcagt ct 22 412 21 DNA Artificial Sequence reverse primer 412 catctgcttc agctcgttgg t 21 413 26 DNA Artificial Sequence probe 413 aagtacacgt aagttacagc cacaca 26 414 18 DNA Artificial Sequence forward primer 414 gcctcggtgt gcctttca 18 415 22 DNA Artificial Sequence probe 415 catcgccagc tacgccctgc tc 22 416 19 DNA Artificial Sequence reverse primer 416 cgtgatgtgc gcaatcatg 19 417 19 DNA Artificial Sequence forward primer 417 gtggatgtgc cctgaagga 19 418 20 DNA Artificial Sequence reverse primer 418 ctgcggatcc agggtaagaa 20 419 28 DNA Artificial Sequence probe 419 aagccaggcg tctacacgag agtctcac 28 420 20 DNA Artificial Sequence forward primer 420 gccctggatt tcagaaagag 20 421 20 DNA Artificial Sequence reverse primer 421 agttacaagc cagggaagga 20 422 25 DNA Artificial Sequence probe 422 caagtctgga tctgggaccc tttcc 25 423 20 DNA Artificial Sequence forward primer 423 ctgctgtctt gggtgcattg 20 424 18 DNA Artificial Sequence reverse primer 424 gcagcctggg accacttg 18 425 25 DNA Artificial Sequence probe 425 ttgccttgct gctctacctc cacca 25 426 19 DNA Artificial Sequence forward primer 426 tgacgatggc ctggagtgt 19 427 22 DNA Artificial Sequence reverse primer 427 ggtaccggat catgaggatc tg 22 428 21 DNA Artificial Sequence probe 428 ctgggcagca ccaagtccgg a 21 429 22 DNA Artificial Sequence forward primer 429 agaggcatcc atgaacttca ca 22 430 24 DNA Artificial Sequence reverse primer 430 caaactccac agtacttggg ttga 24 431 20 DNA Artificial Sequence probe 431 cgggctgcat cagcacacgc 20 432 23 DNA Artificial Sequence forward primer 432 gcagttggaa gacacaggaa agt 23 433 27 DNA Artificial Sequence probe 433 tccccaaatt gcagatttat caacggc 27 434 21 DNA Artificial Sequence reverse primer 434 tgcgtggcac tattttcaag a 21 435 25 DNA Artificial Sequence forward primer 435 agactgtgga gtttgatgtt gttga 25 436 22 DNA Artificial Sequence reverse primer 436 ggaacaccac caggacctgt aa 22 437 23 DNA Artificial Sequence probe 437 ttgctgcctc cgcacccttt tct 23 438 20 DNA Artificial Sequence forward primer 438 acccagtagc aaggagaagc 20 439 20 DNA Artificial Sequence reverse primer 439 cagctggtgg taggttctga 20 440 21 DNA Artificial Sequence probe 440 cactcactgc tccgagtgcg g 21 

What is claimed is:
 1. A method of predicting the likelihood of long-term survival of a breast cancer patient without the recurrence of breast cancer, comprising determining the expression level of one or more prognostic RNA transcripts or their expression products in a breast cancer tissue sample obtained from said patient, normalized against the expression level of all RNA transcripts or their products in said breast cancer tissue sample, or of a reference set of RNA transcripts or their expression products, wherein the prognostic RNA transcript is the transcript of one or more genes selected from the group consisting of: TP53BP2, GRB7, PR, CD68, Bc12, KRT14, IRS1, CTSL, EstR1, Chk1, IGFBP2, BAG1, CEGP1, STK15, GSTM1, FHIT, RIZ1, AIB1, SURV, BBC3, IGF1R, p27, GATA3, ZNF217, EGFR, CD9, MYBL2, HIF1α, pS2, ErbB3, TOP2B, MDM2, RAD51C, KRT19, TS, Her2, KLK10, β-Catenin, γ-Catenin, MCM2, PI3KC2A, IGF1, TBP, CCNB1, FBXO5, and DR5, wherein expression of one or more of GRB7, CD68, CTSL, Chk1, AIB1, CCNB1, MCM2, FBXO5, Her2, STK15, SURV, EGFR, MYBL2, HIF1α, and TS indicates a decreased likelihood of long-term survival without breast cancer recurrence, and the expression of one or more of TP53BP2, PR, Bc12, KRT14, EstR1, IGFBP2, BAG1, CEGP1, KLK10, β-Catenin, γ-Catenin, DR5, PI3KCA2, RAD51C, GSTM1, FHIT, RIZ1, BBC3, TBP, p27, IRS1, IGF1R, GATA3, ZNF217, CD9, pS2, ErbB3, TOP2B, MDM2, IGF1, and KRT19 indicates an increased likelihood of long-term survival without breast cancer recurrence.
 2. The method of claim 1 comprising determining the expression level of at least two of said prognostic RNA transcripts or their expression products.
 3. The method of claim 1 comprising determining the expression level of at least 5 of said prognostic RNA transcripts or their expression products.
 4. The method of claim 1 comprising determining the expression level of at least 10 of said prognostic RNA transcripts or their expression products.
 5. The method of claim 1 comprising determining the expression level of at least 15 of said prognostic transcripts of their expression products.
 6. The method of claim 1 wherein the breast cancer is invasive breast carcinoma.
 7. The method of claim 1 wherein the expression level of one or more prognostic RNA transcripts is determined.
 8. The method of claim 1 wherein said RNA is isolated from a fixed, wax-embedded breast cancer tissue specimen of said patient.
 9. The method of claim 1 wherein said RNA is isolated from core biopsy tissue or fine needle aspirate cells.
 10. An array comprising polynucleotides hybridizing to two or more of the following genes: α-Catenin, AIB1, AKT1, AKT2, β-actin, BAG1, BBC3, Bc12, CCNB1, CCND1, CD68, CD9, CDH1, CEGP1, Chk1, CIAP1, cMet.2, Contig 27882, CTSL, DR5, EGFR, EIF4E, EPHX1, ErbB3, EstR1, FBXO5, FHIT1 FRP1, GAPDH, GATA3, G-Catenin, GRB7, GRO1, GSTM1, GUS, HER2, HIF1A, HNF3A, IGF1R, IGFBP2, KLK10, KRT14, KRT17, KRT18, KRT19, KRT5, Maspin, MCM2, MCM3, MDM2, MMP9, MTA1, MYBL2, P14ARF, p27, P53, PI3KC2A, PR, PRAME, pS2, RAD51C, 3RB1, RIZ1, STK15, STMY3, SURV, TGFA, TOP2B, TP53BP2, TRAIL, TS, upa, VDR, VEGF, and ZNF217.
 11. The array of claim 10 comprising polynucleotides hybridizing to at least 3 of said genes.
 12. The array of claim 10 comprising polynucleotides hybridizing to at least 5 of said genes.
 13. The array of claim 10 comprising polynucleotides hybridizing to at least 10 of said genes.
 14. The array of claim 10 comprising polynucleotides hybridizing to the following genes: TP53BP2, GRB7, PR, CD68, Bc12, KRT14, IRS1, CTSL, EstR1, Chk1, IGFBP2, BAG1, CEGP1, STK15, GSTM1, FHIT, RIZ1, AIB1, SURV, BBC3, IGF1R, p27, GATA3, ZNF217, EGFR, CD9, MYBL2, HIF1α, pS2, RIZ1, ErbB3, TOP2B, MDM2, RAD51C, KRT19, TS, Her2, KLK10, β-Catenin, γ-Catenin, MCM2, PI3KC2A, IGF1, TBP, CCNB1, FBXO5 and DR5.
 15. The array of claim 10 or claim 14 wherein said polynucleotides are cDNAs.
 16. The array of claim 15 wherein said cDNAs are about 500 to 5000 bases long.
 17. The array of claim 10 or claim 14 wherein said polynucleotides are oligonucleotides.
 18. The array of claim 17 wherein said oligonucleotides are about 20 to 80 bases long.
 19. The array of claim 10 or claim 14 wherein the solid surface is glass.
 20. The array of claim 19 which comprises about 330,000 oligonucleotides.
 21. A method of predicting the likelihood of long-term survival of a patient diagnosed with invasive breast cancer, without the recurrence of breast cancer, comprising the steps of: (1) determining the expression levels of the RNA transcripts or the expression products of genes or a gene set selected from the group consisting of (a) TP53BP2, Bc12, BAD, EPHX1, PDGFRβ, DIABLO, XIAP, YB1, CA9, and KRT8; (b) GRB7, CD68, TOP2A, Bc12, DIABLO, CD3, ID1, PPM1D, MCM6, and WISP1; (c) PR, TP53BP2, PRAME, DIABLO, CTSL, IGFBP2, TIMP1, CA9, MMP9, and COX2; (d) CD68, GRB7, TOP2A, Bc12, DIABLO, CD3, ID1, PPM1D, MCM6, and WISP1; (e) Bc12, TP53BP2, BAD, EPHX1, PDGFRβ, DIABLO, XIAP, YB1, CA9, and KRT8; (f) KRT14, KRT5, PRAME, TP53BP2, GUS1, AIB1, MCM3, CCNE1, MCM6, and ID1; (g) PRAME, TP53BP2, EstR1, DIABLO, CTSL, PPM1D, GRB7, DAPK1, BBC3, and VEGFB; (h) CTSL2, GRB7, TOP2A, CCNB1, Bc12, DIABLO, PRAME, EMS1, CA9, and EpCAM; (i) EstR1, TP53BP2, PRAME, DIABLO, CTSL, PPM1D, GRB7, DAPK1, BBC3, and VEGFB; (k) Chk1, PRAME, TP53BP2, GRB7, CA9, CTSL, CCNB1, TOP2A, tumor size, and IGFBP2; (l) IGFBP2, GRB7, PRAME, DIABLO, CTSL, β-Catenin, PPM1D, Chk1, WISP1, and LOT1; (m) HER2, TP53BP2, Bc12, DIABLO, TIMP1, EPHX1, TOP2A, TRAIL, CA9, and AREG; (n) BAG1, TP53BP2, PRAME, IL6, CCNB1, PAI1, AREG, tumor size, CA9, and Ki67; (o) CEGP1, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, STK15, and AKT2, and FGF18; (p) STK15, TP53BP2, PRAME, IL6, CCNE1, AKT2, DIABLO, cMet, CCNE2, and COX2; (q) KLK10, EstR1, TP53BP2, PRAME, DIABLO, CTSL, PPM1D, GRB7, DAPK1, and BBC3; (r) AIB1, TP53BP2, Bc12, DIABLO, TIMP1, CD3, p53, CA9, GRB7, and EPHX1 (s) BBC3, GRB7, CD68, PRAME, TOP2A, CCNB1, EPHX1, CTSL GSTM1, and APC; (t) CD9, GRB7, CD68, TOP2A, Bc12, CCNB1, CD3, DIABLO, ID1, and PPM1D; (w) EGFR, KRT14, GRB7, TOP2A, CCNB1, CTSL, Bc12, TP, KLK10, and CA9; (x) HIF1α, PR, DIABLO, PRAME, Chk1, AKT2, GRB7, CCNE1, TOP2A, and CCNB1; (y) MDM2, TP53BP2, DIABLO, Bc12, AIB1, TIMP1, CD3, p53, CA9, and HER2; (z) MYBL2, TP53BP2, PRAME, IL6, Bc12, DIABLO, CCNE1, EPHX1, TIMP1, and CA9; (aa) p27, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, STK15, AKT2, and ID1; (ab) RAD51, GRB7, CD68, TOP2A, CIAP2, CCNB1, BAG1, IL6, FGFR1, and TP53BP2; (ac) SURV, GRB7, TOP2A, PRAME, CTSL, GSTM1, CCNB1, VDR, CA9; and CCNE2; (ad) TOP2B, TP53BP2, DLABLO, Bc12, TIMP1, AIB1, CA9, p53, KRT8, and BAD; (ae) ZNF217, GRB7, TP53BP2, PRAME, DIABLO, Bc12, COX2, CCNE1, APC4, and β-Catenin, in a breast cancer tissue sample obtained from said patient, normalized against the expression levels of all RNA transcripts or their expression products in said breast cancer tissue sample, or of a reference set of RNA transcripts or their products; (2) subjecting the data obtained in step (1) to statistical analysis; and (3) determining whether the likelihood of said long-term survival has increased or decreased.
 22. A method of predicting the likelihood of long-term survival of a patient diagnosed with estrogen receptor (ER)-positive invasive breast cancer, without the recurrence of breast cancer, comprising the steps of: (1) determining the expression levels of the RNA transcripts or the expression products of genes of a gene set selected from the group consisting of CD68; CTSL; FBXO5; SURV; CCNB1; MCM2; Chk1; MYBL2; HIF1A; cMET; EGFR; TS; STK15, IGFR1; BC12; HNF3A; TP53BP2; GATA3; BBC3; RAD51C; BAG1; IGFBP2; PR; CD9; RB1; EPHX1; CEGP1; TRAIL; DR5; p27; p53; MTA; RIZ1; ErbB3; TOP2B; EIF4E, wherein expression of the following genes in ER-positive cancer is indicative of a reduced likelihood of survival without cancer recurrence following surgery: CD68; CTSL; FBXO5; SURV; CCNB1; MCM2; Chk1; MYBL2; HIF1A; cMET; EGFR; TS; STK15, and wherein expression of the following genes is indicative of a better prognosis for survival without cancer recurrence following surgery: IGFR1; BC12; HNF3A; TP53BP2; GATA3; BBC3; RAD51C; BAG1; IGFBP2; PR; CD9; RB1; EPHX1; CEGP1; TRAIL; DR5; p27; p53; MTA; RIZ1; ErbB3; TOP2B; EIF4E. (2) subjecting the data obtained in step (1) to statistical analysis; and (3) determining whether the likelihood of said long-term survival has increased or decreased.
 23. The method of claim 21 or 22 wherein said statistical analysis is performed by using the Cox Proportional Hazards model.
 24. A method of predicting the likelihood of long-term survival of a patient diagnosed with estrogen receptor (ER)-negative invasive breast cancer, without the recurrence of breast cancer, comprising determining the expression levels of the RNA transcripts or the expression products of genes of the gene set CCND1; UPA; HNF3A; CDH1; Her2; GRB7; AKT1; STMY3; α-Catenin; VDR; GRO1; KT14; KLK10; Maspin, TGFα, and FRP 1, wherein expression of the following genes is indicative of a reduced likelihood of survival without cancer recurrence: CCND1; UPA; HNF3A; CDH1; Her2; GRB7; AKT1; STMY3; α-Catenin; VDR; GRO1, and wherein expression of the following genes is indicative of a better prognosis for survival without cancer recurrence: KT14; KLK10; Maspin, TGFα, and FRP1.
 25. A method of preparing a personalized genomics profile for a patient, comprising the steps of: (a) subjecting RNA extracted from a breast tissue obtained from the patient to gene expression analysis; (b) determining the expression level of one or more genes selected from the breast cancer gene set listed in any one of Tables 1-5, wherein the expression level is normalized against a control gene or genes and optionally is compared to the amount found in a breast cancer reference tissue set; and (c) creating a report summarizing the data obtained by said gene expression analysis.
 26. The method of claim 25, wherein said breast tissue comprises breast cancer cells.
 27. The method of claim 26 wherein said breast tissue is obtained from a fixed, paraffin-embedded biopsy sample.
 28. The method of claim 27 wherein said RNA is fragmented.
 29. The method of claim 25 wherein said report includes prediction of the likelihood of long term survival of the patient.
 30. The method of claim 25 wherein said report includes recommendation for a treatment modality of said patient.
 31. A method for amplification of a gene listed in Tables 5A and B by polymerase chain reaction (PCR), comprising performing said PCR by using an amplicon listed in Tables 5A and B and a primer-probe set listed in Tables 6A-F.
 32. A PCR amplicon listed in Tables 5A and B.
 33. A PCR primer-probe set listed in Tables 6A-F.
 34. A prognostic method comprising: (a) subjecting a sample comprising breast cancer cells obtained from a patient to quantitative analysis of the expression level of the RNA transcript of at least one gene selected from the group consisting of GRB7, CD68, CTSL, Chk1, AIB1, CCNB1, MCM2, FBXO5, Her2, STK15, SURV, EGFR, MYBL2, HIF1α, and TS, or their product, and (b) identifying the patient as likely to have a decreased likelihood of long-term survival without breast cancer recurrence if the normalized expression levels of said gene or genes, or their products, are elevated above a defined expression threshold.
 35. A prognostic method comprising: (a) subjecting a sample comprising breast cancer cells obtained from a patient to quantitative analysis of the expression level of the RNA transcript of at least one gene selected from the group consisting of TP53BP2, PR, Bc12, KRT14, EstR1, IGFBP2, BAG1, CEGP1, KLK10, β-Catenin, γ-Catenin, DR5, PI3KCA2, RAD51C, GSTM1, FHIT, RIZ1, BBC3, TBP, p27, IRS1, IGF1R, GATA3, ZNF217, CD9, pS2, ErbB3, TOP2B, MDM2, IGF1, and KRT19, and (b) identifying the patient as likely to have an increased likelihood of long-term survival without breast cancer recurrence if the normalized expression levels of said gene or genes, or their products, are elevated above a defined expression threshold.
 36. The method of claim 1 wherein the levels of the RNA transcripts of said genes are normalized relative to the mean level of the RNA transcript or the product of two or more housekeeping genes.
 37. The method of claim 34 or 35 wherein the housekeeping genes are selected from the group consisting of glyceraldehyde-3-phosphate dehydrogenase (GAPDH), Cyp1, albumin, actins, tubulins, cyclophilin hypoxantine phosphoribosyltransferase (HRPT), L32, 28S, and 18S.
 38. The method of claim 34 or 35 wherein the sample is subjected to global gene expression analysis of all genes present above the limit of detection.
 39. The method of claim 37 wherein the levels of the RNA transcripts of said genes are normalized relative to the mean signal of the RNA transcripts or the products of all assayed genes or a subset thereof.
 40. The method of claim 38 wherein the level of RNA transcripts is determined by quantitative RT-PCR (qRT-PCR), and the signal is a Ct value.
 41. The method of claim 39 wherein the assayed genes include at least 50 cancer related genes.
 42. The method of claim 39 wherein the assayed genes includes at least 100 cancer related genes.
 43. The method of claim 34 or 35 wherein said patient is human.
 44. The method of claim 42 wherein said sample is a fixed, paraffin-embedded tissue (FPET) sample, or fresh or frozen tissue sample.
 45. The method of claim 42 wherein said sample is a tissue sample from fine needle, core, or other types of biopsy.
 46. The method of claim 42 wherein said quantitative analysis is performed by qRT-PCR.
 47. The method of claim 42 wherein said quantitative analysis is performed by quantifying the products of said genes.
 48. The method of claim 45 wherein said products are quantified by immunohistochemistry or by proteomics technology.
 49. The method of claim 34 further comprising the step of preparing a report indicating that the patient has a decreased likelihood of long-term survival without breast cancer recurrence.
 50. The method of claim 35 further comprising the step of preparing a report indicating that the patient has an increased likelihood of long-term survival without breast cancer recurrence.
 51. A kit comprising one or more of (1) extraction buffer/reagents and protocol; (2) reverse transcription buffer/reagents and protocol; and (3) qPCR buffer/reagents and protocol suitable for performing the method of any one of claims 1, 34 and
 35. 